Preview Software Manual - BioQUEST Curriculum Consortium
Contents
1. Figure 40 A blank plate has no living bacteria Lawn plates see Figure 43 have such a high population of bacteria that there are no distinct colonies only a uniform lawn Lawn plates often arise during serial dilution when tubes with high population densities are plated G Ngee _jo 12345 6 Figure 43 A lawn plate Gridding a Plate To make it easier to read the names of colonies on a plate you can superimpose a grid over the plate by clicking on the grid button in the upper right corner of the plate window The plate in Figure 44 has the grid turned on and the mouse pointer is on the erid button It is legal to replica plate a lawn plate but the results are not realistic No matter what the medium used for the replica the result will be a lawn plate even if none of the bacteria in the lawn should be able to grow on the replica This is a bug Microbial Genetics Construction Kit User Manual 37 Field Plate ee Figure 44 plate with a superimposed grid Shrinking a Plate When you have several plates on the screen you may want to shrink some of them to clear space You can do this by clicking in the close box which is the white rectangle in the upper left hand corner of the window This will cause the plate to shrink to an icon like that shown in Figure 45 Field Plate Figure 45 A plate that has been reduced to an icon To re expand a plate icon double click somewhere on the icon You can select2. Note that the minuses here record complementation not the possibility of growth If B5 is prototrophic for a nutrient it will certainly grow in the absence of that nutrient so if the worksheet recorded growth we might expect to have a at the B5 B5 intersection Microbial Genetics Construction Kit User Manual 49 P1 Penicillin Ss ANGRA BS 2 2 2 2 2 212 2 21212 2 2 ome e EPERE REEEEED erate erate eters erate erate arate eters erate eters erate tsetse erate HE DEOS le le lele wcaele cele HWHH ete BHH tete te sete HEHE erate cele stete te lele HH erate cele lele onene stete HH erate lele lele wraele stete HH erate lele wlele erate cele oe erate lele wlele erate HHA HE erate lele ecele erate stete HH erate lele wlele erate stete HH erate lele ecele cele stete BHH erate lele cele Lele stete HH erate lele erate lele tetet PEPER C C Figure 55 An unfilled out unlocked complementation worksheet for penicillin Controlling a Complementation Worksheet To change the content of a cell click in the cell it will change to the next possible value To change several cells to the same value click and drag across the cells you want to change A worksheet may be locked to prevent accidental changes A locked worksheet is indicated by the closed padlock symbol i in the upper left corner of the window
3. Choose Clean Up on the Utilities menu and pGCK will move all windows back to where they first appeared Quitting This is the end of the tour of Serial Dilution If you want to quit at this point you can do so by choosing the Quit item from the File menu You will be asked if you want to save your work If you decide not to quit after all click on the Cancel button If you save your work the section in the reference section entitled Opening a Saved Problem will tell you how to restore the problem to where you left it If you want more detail on using tubes and plates read the relevant sections of the Reference section If you want a taste of some of the other things that GCK can do read the following Tour sections If you want details on exactly how the computer simulates various aspects of serial dilution read the How pGCK Works section Microbial Genetics Construction Kit User Manual 13 A Tour of Phenotype Identification with GCK This is a tour of phenotype identification with GCK If you just finished a different tour you can choose New Problem from the File menu to start a new problem This is equivalent to starting the program over again The Field Plate You should see a picture of a petri plate similar to that shown in Figure 11 You will have a different number of colonies in different places however so yours will not be identical to Figure 11 Field Plate 2 7 ce G _jo 12345 6 Figure 11 A field pl
4. An unlocked worksheet is indicated by an open padlock symbol To lock an unlocked worksheet or unlock a locked one click on the padlock symbol Shrinking a Complementation Worksheet You may shrink a complementation worksheet to icon form by clicking in the close box see Figure 56 To re expand the icon either double click on it or reselect Complementation Worksheet from the Analysis menu Figure 56 A phenotype worksheet in icon form Filling a Complementation Worksheet 50 Microbial Genetics Construction Kit User Manual Some uGCK problems allow you to fill a complementation worksheet automatically If there is a Fill Complementation Worksheet item on the Analysis menu you can do this Select the complementation worksheet by clicking on its title and then choose the menu item Destroying a Complementation Worksheet To destroy a complementation worksheet select it by clicking on its title and then choose Destroy Worksheet s from the Analysis menu Taking Notes Using Notepads Every plate and tube has an associated notepad to open it click on the notepad icon El in the upper right corner The notepad stays in existence as long as you do not autoclave its associated plate or tube You can close it temporarily by clicking in its close box and when you re open it any notes you typed will still be there Use the notepad just as you would any other Macintosh word processor You can type into it paste pictures
5. Appendix entitled Hardware and Software Requirements p 74 If you are familiar with the Macintosh but not with this program Read one of the sections entitled A Tour of X with uGCK although most of these can be read independently it is best to read each of them in order while working with the program at the same time If you ve been through the Tours of wGCK and want more details Read the section entitled Reference p 37 If you started by skimming the manual but have found something that doesn t seem right Read the section entitled A Word of Warning p 4 the appendix entitled It Doesn t Work p 73 or consult the index p 75 If you are a veteran user of the program and want to know what is different about this version Read the separate document entitled GCK Version History Microbial Genetics Construction Kit User Manual 3 What You Need to Know We assume that you are already familiar with the basic set of standard Macintosh terms and operations If you are not comfortable with these you should read BioQUEST Macintosh Fundamentals or another introduction to the Macintosh before you begin Better yet find someone who knows what she is doing show her this list of words and ask her to explain what each of them means The terms you need to be familiar with are window menu mouse point click shift click drag and double click If you understand these you are ready to get started Before long however you
6. Lawn 10 38 72 Notepad 41 52 Replicate 15 45 Selecting 16 40 Shrink 39 Zoom 39 Plate Tube 46 Plates Icon Form 12 Moving 12 Shrinking 12 Printing Windows 56 Problem Create 60 Delete 60 Edit 60 Name 62 Open 60 Save 58 Prototroph 49 73 Question Mark 57 Quit 12 22 31 Recombination 64 Replica Plating 15 Resistance 49 Restore Problem 60 Save As 59 Save Problem 58 Scrapbook 54 73 Select Tube 43 Selecting Tubes 9 Sensitivity 49 Serial Dilution 7 Setup Problem 60 Shift key 27 56 Simulation Parameters 60 Spreadsheet 55 Strains Number of 62 Tab 55 Time of Entry 64 Tube Autoclave 47 Clear 7 42 Destroy 43 Dilute 45 Diluting 10 Dilution 65 Dilution Factor 42 Field 7 62 History 43 Icon 42 Inoculate 27 Inoculating 46 Notepad 43 Plating 9 46 Selecting 9 43 Shrinking 42 Turbid 7 42 Tubes Icon Form 12 Moving 12 Shrinking 12 Window Printing 56 Word Processor 52 54 55 Worksheet Close 22 Complementation 29 50 65 Destroy 50 Filling 50 52 Icon 22 50 Locking 25 31 50 Organizing 25 Phenotype 20 24 48 65 Shrinking 22 50
7. Manual If you click on the button labeled Cancel instead of Start Problem GCK will stop running Once you have selected a problem proceed to the section describing the closest tour Microbial Genetics Construction Kit User Manual 7 A Tour of Serial Dilution with GCK The Field Tube You should see a picture of a test tube like that shown in Figure 3 This test tube is filled with an unknown number of bacteria of unknown phenotype and genetic makeup The test tube is referred to as the Field Tube because it represents a set of bacteria collected from the field In this tour of serial dilution we will look only at the number of bacteria the bacterial phenotypes and genetic makeup will be examined elsewhere The critical thing to note about this test tube is that it is light gray This indicates that the tube is turbid It has enough bacteria in it to scatter light Soon we will see tubes that are clear indicating that they have far fewer bacteria Figure 3 A field tube Serial dilution is a process of preparing increasingly dilute populations of bacteria until the population is small enough to be counted by hand Individual bacteria can t be counted easily because they can t be seen An easy way to count bacteria is to put them on a petri plate let them grow and count the colonies that result from the individual bacteria If there are too many bacteria this will not work because we won t be able to tell which colonies result from
8. Microbial Genetics Construction Kit User Manual entire computer screen will be printed These procedures are not only part of GCK but are characteristic of every Macintosh program Getting Help There are several ways to ask for help from pGCK or any other BioQUEST program Why Can t Use This Menu Item At any one time several menu items will be gray indicating that they are inactive and therefore cannot be used Active menu items appear in black It is not always obvious why a menu item is inactive or how to make it active In pGCK if you try to choose an inactive menu item you will get a short message explaining what to do in order to enable it see Figure 56 Usually this means selecting an object Plate Replicate In order to use this option you must first select 4 petri dish select 4 dish by clicking ina spot where there is no colony If there are no petri dishes on the Cancel Figure 58 A Help message explaining why the Replicate Plate item is inactive Use the scroll bar on the right to see text that is not immediately visible When you have finished reading the help message you can dismiss it by clicking on the Cancel button What Is This Thing For To find out something is or does you need to be in help mode To enter help mode press the command key while simultaneously pressing the question mark key On some keyboards there is a key labeled help If your keyboard has a help key it will do the s
9. Terry L Derting Murray State University Roscoe Giles Boston University Louis Gross University of Tennessee Knoxville Yaffa Grossman Beloit College Raquel Holmes Boston University Stacey Kiser Lane Community College Peter Lockhart Massey University NZ Ed Louis The University of Nottingham UK Claudia Neuhauser University of Minnesota Patti Soderberg Conserve School Daniel Udovic University of Oregon Rama Viswanathan Beloit College Linda Weinland Edison College Anton Weisstein Truman University Richard Wilson Emeritus Rockhurst College William Wimsatt University of Chicago Copyright 1993 2006 by John N Calley and John R Jungck All rights reserved Copyright Trademark and License Acknowledgments Portions of the BioQUEST Library are copyrighted by Annenberg CPB Apple Computer Inc Beloit College Claris Corporation Microsoft Corporation and the authors of individually titled modules All rights reserved System 6 System 7 System 8 Mac OS 8 Finder and SimpleText are trademarks of Apple Computer Incorporated HyperCard and HyperTalk MultiFinder QuickTime Apple Mac Macintosh Power Macintosh LaserWriter ImageWriter and the Apple logo are registered trademarks of Apple Computer Incorporated Claris and HyperCard Player 2 1 are registered trademarks of Claris Corporation Extend is a trademark of Imagine That Incorporated Adobe Acrobat and PageMaker are trademarks of Adobe Systems Incorporated Microsoft Wi
10. The ability to change parts of the program to better fit your needs and instructional objectives In GCK you can change the set of operations available on the menu bar the range of genetic phenomena that occur in a problem and the names of the traits and variations used by the program A window that contains requests for instructions or information For instructions on using dialog boxes see your Macintosh Owner s Guide The population of the first vial to appear on the screen This population was collected from the field and is not the result of a cross so its phenotypic ratios are not significant Microbial Genetics Construction Kit this program A group of bacteria with the same genotype A plate without distinguishable colonies because of overlap At the very top of your Macintosh computer screen there is a white bar with a number of symbols and words This is called the menu bar and each of the symbols and words is the title of a menu For more information about menus and how to use them see your Macintosh Owner s Guide Please see your Macintosh Owner s Guide for information about what a mouse is and how you use it A notepad is a window that you can type into or insert pictures into It is a place to write notes to yourself or to collect your thoughts for a lab report Each plate and tube has a associated notepad To open it click on the E symbol in the upper left of the vial When we use the word object in this manua
11. automatically select the new tube for you to make it easy to plate it or dilute it again Automatic Tube Dilution Many pGCK problems are set up so that tubes are automatically diluted when they are plated In these problems the Dilute 10 Fold option will probably not exist In some problems there may be a Dilute Automatically option on the Tube menu which allows you to turn automatic dilution on or off If there is a check mark V next to the Dilute Automatically option it is turned on Plating a Tube There are three ways to plate a tube depending on what medium you want to use for the new plate To use any of them select the tube and then choose the appropriate option from the Tube menu Plating a tube behaves differently depending on whether pGCK has been configured to automatically dilute tubes before plating If not the resulting plate may be a lawn or 44 Microbial Genetics Construction Kit User Manual blank depending on the number of bacteria present in the tube For descriptions of what this means see the section entitled Reading a Plate If automatic dilution is turned on the tube s concentration will automatically be lowered so that the plate has distinct colonies if possible The required dilution will be recorded in the tube s notepad Plate Tube on Tube Medium This will create a new plate using a copy of the nutritional medium used in the tube Plate Tube on New Medium This will ask you to construct the medium to be
12. material from one program into the clipboard switching to the other program and then Pasting the clipboard into the second program This can be quite clumsy if you need to move several different things between the same two programs since the clipboard can only hold one thing at a time In this situation you may want to look into using the Macintosh Scrapbook see your Macintosh Owner s Guide which can hold more than one thing at a time Cut Copy Paste and Clear You can use Cut Copy and Paste to move text and pictures between GCK notepads and other programs Unfortunately however it is not possible to copy and paste mixed text and pictures at one time To copy a notepad that contains both text and pictures you need to do the following Microbial Genetics Construction Kit User Manual 53 Select the entire content of the notepad You can do this by clicking before the first word and dragging to the end or by clicking once before the first word scrolling to the end and shift clicking after the last character Choose Copy from the Edit menu Paste the result into an external word processor Where pictures exist in the original notepad you will see a little box For each picture in the notepad Select the picture Itis critical that you select only the picture and no surrounding blank space Choose Copy to put a copy of the picture on the clipboard Paste the picture into your word processor Copy Win
13. nigh Ge 0 qi acme nrenrree E E 11 TS posses E EE E N EEEE E EEEE 11 Rearranging Plates and TUDeS esnie iio 11 SOTUKING llates AiG TUDES eie nia po isins iin 11 A IR en EE EAEE EE 12 RT ec csp E cee gee aes oes ea seco op cease sp cage oar eeqsediasenaesteeeae gees 12 A Tour of Phenotype Identification with GCK oe eee ceeeseeseeeeeeeeeeeeaeens 13 Toe gts Ce Plil Essun eran Cerne een er eer tr ere ee E en 13 TR FS Pa ee pact E cera mee EA A E E A 14 7s 0 0d HE eg o EE E E EEA 14 CC a E le r A TE usadersoumeconnsvccsennendeeaaeo 15 Peer a NTE Ta E E E 15 PI E E E E toca sepeeseeeinaasia 17 Checking the Mediti seipsos ien rara norin EER roren En TER EEPE RNE EO 18 Bord Te RE U n a E E E EEEE EE E E EEE 19 Opena Phenotype Worksheet suscipe i oS 19 Close the Works heti ce ssite oragide sue ao cnarrau ni E ge 21 RIE E E E E E a ace eens 21 A Tour of Complementation Testing with GCK seeesseseeseerserssrsrrsrrsrrrrsresrrsreereeess 22 Te e I Ve e e E E E A E N E E E iS 22 Looking at Colony T henoly eS svcisisesosensaczenrseniowsscnnnmarceyedevisranumivusvenaventuanees 23 Organizine the ENCHOLY DES contsoncsrhatean coamatinenansnasanceoscantetebessndtentianneasaduensean 24 Tecan FOr CSS FCC cpt cn ne sees E A 26 TREC ORCS TS IRS S CS ena a E E E A 28 ROSIN ois soca eos crsag acces E E E cig ee aegis ee aaeg ees 30 A Tour of Conjugation Mapping with PGCK eee eeecereeeeeeneeeeeneeees 31 Looking at Colony Phenotypes sorsra pa e En Enan e 31
14. oclecUng Colonies tO COn Ugal Oeser erin 31 Ca O aa E EE E A A E AA E 32 Plating the Conjugate Population cece ee cess eceeeeeeeeseeeeeenseeeeeees 33 DIET oe asc asst E E E se acaootounenengn scare uated econ ces 34 Ketere NCE sierran ca ueamnetnemarasree E E AEE OE stat 35 TRAC eB VAS reste stato E E A E O E 35 Ca aT AO a E A E 36 Salaa eae a e E A E A E 37 Aea e E a e E E spn aenrauncasneesecsseetonciaeer 37 SNS CANS VALS A E selovessvesatastasevaes 38 Take Notes oma Pate vais sect isien EET iE AAEE 39 Getting the History of a Plate eeeseeseseeseesseerrersrrsrrsrsrrsrrsresrrsrreeses 39 POO CS a laers oenn E S 39 pE a A T E a dacesneoeceiystyveayesseso qadmerudoreaaessek aera oeaor semen 39 keadinie a TUDO upire i nnr eee E E E 40 Pena AL DG eaea E E E 40 Celec ne a I ODO EEEE 41 DE aE A 0 e T E T 41 Getting the History of a Tube ssessessesseeseeresrssrsresrrsresrsrrsresresresrreeses 41 a AT o EE E E TE 41 ROMS EEG U ES Medid asetin Erienn eE E EESO A E E 41 Exp orien a OS ae E E EE 43 Keplica Plating a TNA te cress ssseutaarerassosnasiso se inasssansemsmnoactvauniseieviebotioatannines 43 Experiments With TUDES seise pinssss kisii arinn E E NE EEEE 43 Dauti A LUD eon a e A A A E E E E 43 Automatic Tube Dilution eessessessssesserseesersesseserseeseeseeeeseesees 43 Paunga TUD Oae a A E E S e EE 44 Experiments WNC O1OM 16S sesepan EE 44 TNO CONAN a TADE eaa EA E E 44 SOM GI TWO E S E E eotenseern cunt saueanees 45
15. save your work the section in the reference section entitled Opening a Saved Problem will tell you how to restore the problem to where you left it If you want more detail on using plates tubes and worksheets read the relevant sections of the Reference section If you want a taste of some of the other things that GCK can do read the other Tour sections If you want details on exactly how the computer simulates various aspects of conjugation read the How GCK Works section Microbial Genetics Construction Kit User Manual 35 Reference Plates Notepad foom box Close box tuttan Field Flate TON A7 E AKRI Ilk Figure 40 The parts of a plate Reading a Plate uGCK plates may be blank have colonies or have a bacterial lawn Most plates created while working with pGCK have one or more colonies and look somewhat like Figure 41 Each of these colonies represents an isogenic strain of bacteria Colonies are identified by row letter and column number The pointer in Figure 41 is on colony G2 fjeld Plate 2 lo 123 45 6 Figure 41 A plate with 18 colonies Blank plates see Figure 42 result from plating tubes with very small populations or from plating a tube onto a plate with media that does not allow any bacteria to grow 36 Microbial Genetics Construction Kit User Manual In any case blank plates have no living bacteria Although it is possible to replica plate a blank plate only blank plates will result
16. ten since one tenth of the tube s volume was put on the plate Since there are 35 colonies our first approximation of the population in the field tube is 350 million bacteria 35 times 10 times 109 Once you have a diluted tube that yields a countable number of colonies plate it several times and compare the results Try diluting it again and then plating it Cleaning up Depending on how you chose to do things you probably have eight or nine tubes and five or six plates by this time and the screen is getting pretty crowded uGCK provides a number of aids help clean things up Rearranging Plates and Tubes Petri plates and test tubes are normal Macintosh windows and you can drag them just as you drag most other windows This is a way to manually clean things up Shrinking Plates and Tubes Most of the plates and tubes you produced during the preceding exercise aren t intrinsically very interesting You can shrink close them to get them out of the way and concentrate on the interesting ones To close a plate or tube click in the white box in the upper left hand corner of the window the mouse arrow is in the close box in Figure 9 Figure 10 shows icon versions of a plate and a field tube 12 Microbial Genetics Construction Kit User Manual Plate 3 Field Figure 10 Icon forms of a test tube and a petri dish To re expand open one of these icons double click on it Asking GCK You can also ask pGCK to clean things up for you
17. used for the new plate Plate Tube on Last Medium This will create a new plate using the same medium that was used to create the last plate Experiments with Colonies Inoculating a Tube You can inoculate a tube with one or more colonies by selecting the colonies and choosing one of the three Inoculate Tube options from the Colony menu To select a colony click on it to select more than one colony hold down the shift key while clicking The colonies you select may be on one or several plates When you inoculate a tube with a set of colonies GCK will put equal quantities of each strain of bacteria into a new tube and incubate the tube If all strains are equally able to grow in the tube medium they will be present in equal proportions If one or more strains cannot grow it will not be noticeably present in the final population of the tube In pGCK all intermediates in a biochemical pathway cistron products can diffuse through cell walls If two auxotrophic strains are grown together in a liquid medium they will complement if their defects are on different cistrons If the defects are on the same cistron complementation will not occur Inoculating a tube with a population containing both Hfr and F strains will not result in any conjugation To conjugate two strains you must explicitly request conjugation Inoculate Tube in Plate Medium This will create a new tube that contains the same nutritional medium as that used in the plate
18. which individual bacteria If there are only a few bacteria on the plate however there will only be a few colonies and we can tell how many individual bacteria were on the plate before the growth In order to do this we need to be able to put the bacteria that are in a tube on a petri plate and let them grow This is called plating a tube 8 Microbial Genetics Construction Kit User Manual Plating a Tube Get Some Help Edit inte Tee Utilities Hiteda tf faid srira Parke fir Eo Peel SR CEREEYT ERG Bb Dany ds Sitiidi Pfhige pfp ure 4 The Tube menu In Figure 4 the Tube menu has been pulled down You can see that the menu itself and all of the menu items are gray A menu is gray if all of its items are gray and a menu item is gray if it won t do anything A gray menu or menu item is usually called inactive In GCK if you try to choose an inactive menu item you will be shown a short message explaining why the item is inactive and how to make it active To try this pull down the Tube menu and try to choose the Plate Tube on Tube Medium menu item When you release the mouse button a window like that in Figure 5 will appear To see the remaining text move the mouse pointer over the downward pointing arrow and click To dismiss the help message click on the Cancel button Tube Plate Tube On Tube Medium In order to use this option you must first select a test tube lf there is a test tube on the screen you can
19. will also need to know several more Macintosh vocabulary words close box zoom box grow box title bar scroll bar clipboard and desk accessory We also assume that you know how to start a program If you think you know how but you experience some difficulty look at the Appendix entitled It Doesn t Work for suggestions that we hope will help 4 Microbial Genetics Construction Kit User Manual A Word of Warning It is possible that what you read in this manual may not accurately reflect what you see on the screen as you use the program There are two basic reasons for this First uGCK is not yet a final product It is changing as we improve it and add new capabilities The manual you are reading may have been written to go with a different version of the program than the one you are using If you suspect that this may be the case refer to the Appendix entitled It Doesn t Work It will tell you how to check for this problem The second reason for a conflict between the manual and the program is intrinsic to the design of GCK itself We have tried to make pGCK a flexible program so that it can be adapted to fit the needs of many situations We feel that this is a good thing but it makes describing the program a bit difficult There are several differences that may be due to customization of the program The menus we describe here may be different from yours In particular it is possible that a menu operation that we describe may b
20. your observations about colony phenotypes or display the phenotypes automatically Opening a Phenotype Worksheet To open a phenotype worksheet choose the Phenotype Worksheet from the Analysis menu If there is only one possible phenotype worksheet because there is only one plate or because all plates are derived from one plate by replica plating the menu item will always be active If there are two or more possible different phenotype worksheets you need to select the plate before choosing the menu item Reading a Phenotype Worksheet Phenotype worksheets record the phenotypes of the colonies listed along the top with respect to the categories listed along the left The title of the phenotype worksheet indicates which plate the colonies come from in Figure 53 the P1 refers to Plate 1 The first line shown in Figure 53 may be displayed if the status of the F plasmid is significant for a problem If it is displayed Hf indicates that the colony is an Hfr strain has the F plasmid integrated into its chromosome F indicates that the strain does not contain the F plasmid and indicates that its status is unknown Nutrient synthesis ability is indicated by a if the strain is prototrophic can synthesize the nutrient a if it is auxotrophic cannot synthesize the nutrient or a if its status is unknown Antibiotic resistance is indicated by an r if the strain is resistant to the antibiotic an s if it is sensitive to the antibioti
21. Analyzing and Organizing Your Data e eessessessesserserseesersersrssessreseserseeseeses 45 MEM N a E E E R 45 PHENO pE VV OP KSI CUS sineren E E 46 Opening a Phenotype Worksheet sessssessesssssssseseeseeseesess 46 Reading a Phenotype Worksheet cccce cece eee ceeeeeenees 46 Controlling a Phenotype Worksheet c ee eeeeeeeeeeeee 47 Shrinking a Phenotype Worksheet eee eeeeeeeee 48 Filling a Phenotype Worksheet cccceceeseceeeseeeeeeeeeeeees 48 Destroying a Phenotype Worksheet 48 Complementation Worksheets cesses eeseeseseeseeeeeeeneens 48 Opening a Complementation Worksheet 48 Reading a Complementation Worksheet c cece eee 48 Controlling a Complementation Worksheet 0 49 Shrinking a Complementation Worksheet 49 Filling a Complementation Worksheet cee eee 50 Destroying a Complementation Worksheet 50 Taking NOIES scieneo senise nennir a ea EEEE EE ENEN TESE EEEa 50 UE NOE AS e E E 50 Penti NoE E E RA E E I AE 51 Cleaning Up ihe BEnchiOp seesi ieai E E RR 51 Changing the Cleanup ProOCOSS iscissi eanne 51 Communicating With Other ProgramS essessserserserseresresreseessrseersesereseeses 92 C t Copy Paste and Cleat ep mene nee eae enn One ene mere rere 52 COPY NINGUN aee rrr ter errr er E ner er tert ee 53 OY N OW Dai i a EERE 53 Penuaan E A EEE 54 Cera nE e EA E E A oa Saba A TE 54 Why Can t I Use This Menu Item sssesse
22. Microbial Genetics Construction Kit GCK Version 1 B0 7 User s Manual BioQUEST 4 ay i 2 A e 3 ae ch iy sr Library VH TA John N Calley University of Arizona John R Jungck Beloit College A BioQUEST Library VII Online module published by the BOQUEST Curriculum Consortium The BioQUEST Curriculum Consortium 1986 actively supports educators interested in the reform of undergraduate biology and engages in the collaborative development of curricula We encourage the use of simulations databases and tools to construct learning environments where students are able to engage in activities like those of practicing scientists Email bioguest beloit edu Website http bioquest org Editorial Staff Editor Managing Editor Associate Editors John R Jungck Ethel D Stanley Sam Donovan Stephen Everse Marion Fass Margaret Waterman Ethel D Stanley Amanda Everse Sue Risseeuw Online Editor Editorial Assistant Beloit College Beloit College BioQUEST Curriculum Consortium University of Pittsburgh University of Vermont Beloit College Southeast Missouri State University Beloit College BioOQUEST Curriculum Consortium Beloit College BiOQUEST Curriculum Consortium Beloit College BioQUEST Curriculum Consortium Editorial Board Ken Brown University of Technology Sydney AU Joyce Cadwallader St Mary of the Woods College Eloise Carter Oxford College Angelo Collins Knowles Science Teaching Foundation
23. S VU Sie DUN recre E E E E 73 Hardware and Software Requirements esessesesserseserseesrssrsesreseesesseseesesees 73 What is Microbial Genetics Construction Kit Microbial Genetics Construction Kit uGCK is a simulation of a microbial genetics laboratory It provides you with a set of unknown bacteria on a petri plate or in a test tube You can then investigate many of the characteristics of these bacteria using tools similar to those used in a real laboratory GCK is not meant to replace work with real organisms But the constraints of time space money and unskilled laboratory technique important parts of real scientific research make it practically impossible for most students to experience the excitement and challenge of a real research problem uGCK can give you the chance to work with problems that have the real surprise and real complexity that make scientific research a fascinating activity We have tried in this program to let you tackle realistic problems in a way similar to that used in real scientific research You or your instructor however can set up GCK so you can start with a simplified world and add new material as your understanding grows 2 Microbial Genetics Construction Kit User Manual What You Should Read If you are unfamiliar with the Macintosh computer Read the separate document BioQUEST Macintosh Fundamentals If you want to know whether or not you have the right equipment to run the program Read the
24. SAS SS SSS SS SS a AA T PEE AN PEE AN PEE N AAAs Ce CA ga ae a a C a a a ros ne 0 0 0 PPP PP AAAA AALA S FOR BOS A x S JM r x ACACA 5 55 CALA re TAS S AAA Ge S o CRRA x Psy vai es FARR 0 n EEEE 7 645 FSS tute Lat af aaa ut FFF tut es FFF tutes a a nT ore a PEIN PEIE AIN Q Q DAE ALAA AA CACARACA oe ee 5 x DOCE DOCO SAS SS rd oe a a CELE PEE EEES PE A PEE a AA a a a a CAAA AAA CAAA a P P x ee Pe ee ee TASS er rd oe SADAAASS o Pees rs GT ares A A Ft Onn a ea a On a a aa a Py Py Py Ay Py Py Py ee Py Py Ay Fy ee Py Py Py Py ee AAAA SRO OOO ALAARA PIIN Cours 5 ae AS rs Peay PIIN TAADPASAS Figure 52 The media matrix The rows of the media matrix record the presence or absence of the nutritional factors and antibiotics named The columns name the plates and tubes referred to In the media matrix shown in Figure 52 plate 3 is shown to have the nutritional factors alanine tyrosine and biotin 46 Microbial Genetics Construction Kit User Manual You may reorganize the media matrix to bring items of interest together by dragging rows and columns To drag a row or column place the mouse pointer on the name of the row or column and drag the dotted outline to the desired position Phenotype Worksheets Phenotype worksheets record the phenotypes of colonies Depending on the way that uGCK is set up they either provide a place for you to record
25. ala tyr bacteria D2 is an F colony of ala tyr bacteria To select two colonies click on one of them and then click on the second colony while holding down the shift key 32 Microbial Genetics Construction Kit User Manual Field Plate T oa 23456 Figure 35 Sa field plate with colonies A2 and D2 selected Conjugating Once you have selected two colonies choose Conjugate from the Colony menu The window shown in Figure 36 will open for you to enter the conjugation time 1 Grow both colonies independently 2 Combine the populations and incubate them together for minutes 4 Agitate the tube to break up pairs Figure 36 Choosing the conjugation time Click on the OK button to start conjugating When GCK is finished with the conjugation it may take some time it will create a tube filled with the conjugate population see Figure 37 This tube is created with a complete nutritional medium Microbial Genetics Construction Kit User Manual 33 Figure 37 A tube full of conjugant bacteria Plating the Conjugate Population The tube that results from the conjugation has a combined population of parental bacteria and any recombinants from the conjugation To see if the conjugation has produced any recombinants at the alanine locus we need to plate the tube on a restrictive medium that will not allow either of the parental strains to grow To plate the tube select it and choose the Plate Tube on New Medium opti
26. always be a Cancel button Pressing it will close the help window There will often be a Back button as well Pressing it will return you to the topic list that led you to the current window Sometimes there will be other buttons that should be labeled so as to be self explanatory S ESK Help SE Using HELP What is GCK Objects and Operations Petri Plates Test Tubes worksheets Saving Loading Problems Cancel Figure 60 The Help with pGCK topic list Clicking Open will lead to information about saving and restoring problems Saving and Opening a Problem Saving a Problem You can save the state of the problem you are working on at any point by choosing the Save option from the File menu This saves everything so that you can later come back to the problem in the same state it was in when you left it There are a number of reasons you may want to save a problem The simplest is that you may want to take a break and come back to a problem later Another reason is to keep all of your original research data If someone then challenges your conclusions you can go back to the original organisms with new questions Or you may want to Microbial Genetics Construction Kit User Manual 57 save a copy of a problem before you do any work at all so that another research team can work on exactly the same problem and you can pool and argue over your results You may also want to save against the possibility of catastrophe in the form o
27. ame thing f When you are in help mode the mouse cursor will look like this instead of the usual arrow shape In help mode all menu items are always active Selecting a menu item will give you a short description of what the menu item does see Figure 59 Microbial Genetics Construction Kit User Manual 55 Plate Replicate This option allows you to replicate 4 plate onto another plate with different media This allows you to isolate the nutritional requirements of the colonies on the plate Figure 59 An Explanation of the Replicate Plate menu item Besides menus you can click on just about anything and get some information about it Usually you automatically drop out of help mode after you get help once Sometimes you want to ask for help on several things and it is useful to stay in help mode If you hold down the option key while clicking you will stay in help mode 56 Microbial Genetics Construction Kit User Manual What About the Big Picture The general help system is accessible from the Help With GCK option under the Apple menu If you choose this option you will be given a list of topics from which to choose the subject of interest see figure 60 To open a topic click on it and click the Open button at the bottom of the help window or double click on the topic line When you open a topic you will either see a list of sub topics or a discussion of the subject At the bottom of a help window there will
28. ate Figure 11 shows a field plate Each of the gray circles represents one colony The idea is that the colonies shown on the plate were grown from bacteria collected from the field and are presented here for your analysis The colonies are of unknown genotype and phenotype although all bacteria within a colony share a genotype and phenotype The letters along the left side and the numbers along the bottom of the plate form a erid that is used to name the colonies The single colony in the top row for example is referred to as colony A4 To make the grid easier to read you can draw all the grid lines by clicking on the grid button which is the set of cross hatched lines in the upper right hand corner of the window In Figure 12 the mouse arrow is shown over the grid button 14 Microbial Genetics Construction Kit User Manual Field Plate 2 Fe EEEN el LL jo1i123456 Figure 12 A gridded plate The mouse arrow is over the grid button Figure 12 shows a plate after the grid has been turned on To turn the grid back off click on the grid button again Replica Plating Replica plating is a method of copying bacteria from one plate to another plate while maintaining the relative positions of colonies By changing the growth media used on the new plates you can infer colonies nutritional requirements Get some Help Bote Analysis He ERELR EECA k s Pies His dais oe gure 13 The Plate menu When you pull down the P
29. be different for every nutrient you need to specify which to use Figure 32 shows how to select a nutrient Click on the name of the nutrient you want and click the OK button Microbial Genetics Construction Kit User Manual 29 Please choose a nutrient for this complementation worksheet Alanine Thiamine Riboflavine Niacin Tyrosine Penicillin Rifamycin Figure 32 Choosing a nutrient for a complementation worksheet The rows and columns of a complementation worksheet are both labeled with the names of the colonies on the field plate The cells at the intersections of rows and columns record whether or not the corresponding colonies complement each other You will notice in Figure 33 that most cells are filled with question marks to show that their complementation status is unknown Those cells that record the complementation of a colony with itself however are automatically filled with minuses since colonies cannot complement themselves We know that colonies C4 and C6 do not complement We can record this information by clicking twice at the intersection of row C4 and column C6 or vice versa The first click changes the cell to a plus which would indicate complementation The second click changes the cell to a minus The mouse pointer in Figure 33 is pointing at the intersection of row C4 and column C6 30 Microbial Genetics Construction Kit User Manual P1 Alanine 4 eeeeleeleeleele ele p1 tel leteleletele
30. c or a if its status is unknown Microbial Genetics Construction Kit User Manual 47 P1 Phenotypes Alanine Biotin Figure 53 A filled in and locked phenotype worksheet with a plasmid row Controlling a Phenotype Worksheet To change the content of a cell click in the cell it will change to the next possible value To change several cells to the same value click and drag across the cells you want to change A worksheet may be locked to prevent accidental changes to its contents A locked worksheet is indicated by the closed padlock symbol i in the upper left corner of the window An unlocked worksheet is indicated by an open padlock symbol i To lock an unlocked worksheet or unlock a locked one click on the padlock symbol Shrinking a Phenotype Worksheet You may shrink a phenotype worksheet to icon form by clicking in the close box see Figure 54 To re expand the icon either double click on it or reselect Phenotype Worksheet from the Analysis menu P1 Phenotypes Figure 54 A phenotype worksheet in icon form Filling a Phenotype Worksheet Some uGCK problems allow you to fill a phenotype worksheet automatically If there is a Fill Phenotype Worksheet item on the Analysis menu you can do this Select the phenotype worksheet by clicking on its title and then choose the menu item 48 Microbial Genetics Construction Kit User Manual Destroying a Ph
31. corner of the window To relock click again If we were recording antibiotic resistance we would click in the antibiotic rows at the bottom of the worksheet to switch between r resistant s Sensitive and unknown P Phenotypes Alanine anine rao Pelate Biotin ielelelelelelelelelelelele eel Thieming lelelelelelelee Peele eer inortavind 2 2 el lelelelelelelelelel Niacin efofetetotel otetol etetol ef etol TIT IL PLP el ele lel el Figure 22 A phenotype worksheet with the alanine status of colonies A4 B4 and B5 Close the Worksheet To close the worksheet click in the close box in the upper left corner The worksheet will collapse to a small icon see figure 23 You can re expand the worksheet by double clicking on the icon or by re choosing the Phenotype Worksheet item on the Plate menu Microbial Genetics Construction Kit User Manual 21 RPR tias nnn os ee ser P1 Phenotypes Figure 23 A collapsed phenotype worksheet Quitting This is the end of the tour of Phenotype Identification If you want to quit at this point you can do so by choosing the Quit item from the File menu You will be asked if you want to save your work If you decide not to quit after all click on the Cancel button If you save your work the section in the reference section entitled Opening a Saved Problem will tell you how to restore the problem to where you left it If you want more detail on using pla
32. dentical to this one because your field plate is different The columns are labeled across the top with the names of colonies on the field plate The rows are labeled along the left side with the names of the available nutrients and antibiotics To find the relationship between a colony and a particular nutrient look at the cell at the intersection of the appropriate row and column Remember that a plus sign indicates prototrophy or that the colony does not require that nutrient in order to grow A minus sign indicates that the colony is auxotrophic for the nutrient so it requires it to grow For antibiotics an r indicates resistance and an s indicates sensitivity If you went through the previous tour you know that you can click on a worksheet cell to change its contents This will not work in this example because this worksheet has been locked to prevent accidental changes You can unlock a worksheet by clicking on the padlock button i in the upper left corner of the window To relock click again Organizing the Phenotypes We will be doing complementation testing between auxotrophs for the same nutrient to see if their defects are sufficiently different that they complement each other For our purposes then nutrients for which we have few or no auxotrophic colonies are not interesting It is nice in cases like this to be able to forget about the uninteresting nutrients and concentrate on those that are more immediately usef
33. dow The Copy Window option on the Edit menu is always active as long as there is at least one window open It will put a picture of the current frontmost window on the clipboard Once it is on the clipboard it can be pasted into a notepad or into another Macintosh program The picture of the window looks exactly like the window This is potentially confusing because it is not a window any more but just a picture of one This means that the close box and other controls will not work Copy Window Data The Copy Window Data option on the Edit menu will put a copy of the data a window contains on the clipboard in a form that is usable not only displayable by other programs The data is in tab delimited text format that is usable by many word processors spreadsheets data base managers and graphing programs Tab delimited text is text arranged in columns with each column separated by a tab If you paste this into a word processor you will need to set the tab stops to line up the columns The media matrix phenotype worksheets and complementation worksheets are the uGCK windows that export their data in this way The data stored in the frontmost window will be exported Printing a Window You can always print the frontmost window if you have a printer attached to your computer by holding down three keys simultaneously The three keys are the shift key the command key and the 4 key If you also press the caps lock key the 54
34. e missing in your problem We strongly recommend that you use the version of GCK with the tour problems and use the problem appropriate to the tour you are reading so you won t run into this The genetic organization of the bacterial species will be different every time you run the program The set of nutrients and antibiotics used may be different At the moment you cannot change this yourself but we have built two versions of uGCK one with a long list of nutrients and one with a short list Eventually you will be able to change this yourself Microbial Genetics Construction Kit User Manual 5 Getting Started Starting the Program To start the program double click on the GCK program icon see Figure 1 Figure 1 The GCK program icon The next thing you see will be a list of problems such as that shown in Figure 2 If you are taking the first tour Serial Dilution you will want to choose the first problem Choosing a Problem RIGGS CONST UGTION RIT Version 1 60 4 Please choose a problem Serial Dilution Tour Phenotype Identification Tou Complementation Tour Conjugation Tour Full Menus Start Problem Figure 2 Selecting a GCK problem To choose a problem click on it to highlight it in black like Serial Dilution Tour in Figure 2 then click on Start Problem If you don t have exactly this list of problems choose one that seems similar to one of those listed 6 Microbial Genetics Construction Kit User
35. edit GCK problems you must have access to a copy of GCK with the Edit Problem Types option under the Utilities menu Most copies of GCK have this capability disabled so as to prevent users from looking at the description of the problem they are trying to solve If you choose Edit Problem Types you will first be presented with a list of the available problems and given an opportunity to delete a problem to create a new problem or to open and edit a currently existing problem see Figure 63 Which problem type Serial Dilution Phenotype Identification Complementation Conjugation Full Menus pelete Figure 63 Choosing a problem type to change or delete or creating a new problem type Once you have selected a problem to work on you will be given an opportunity to change the problem type s name to change the field population parameters to change the genome configuration or to modify the problem menus see Figure 64 Microbial Genetics Construction Kit User Manual 59 Problem Type Name Serial Dilution Click on the parameter set you wish to change Field Population Genome Configuration Menu Options Cancel Figure 64 Change problem type name and select parameters to change You can edit the problem type name with the normal Macintosh text editing techniques To edit one of the parameter sets click on the appropriate button Field Population Parameters O Field Plate Field Tube Number of strains Minim
36. enome Configuration Length of bacterial chromosome minutes Number of markers Minimum Mian nimum Cistrons per marker Minimum i Ma simum a Beads per cistron Minimum Ma imum Marker Distribution Auxotrophic Resistant To Degradative o To Conjugation Model Time of Entry O Recombination Figure 66 Genome Configuration editing Microbial Genetics Construction Kit User Manual 61 Length The first line allows you to set the length of the bacterial chromosome in minutes Make it smaller for a chromosome more densely populated with markers This is also significant for conjugation Longer chromosomes will lengthen the time required for conjugation Markers The second line sets the size of the universe of possible markers from which subsets will be drawn and assigned to particular strains In Figure 66 we have decreed that there be seven possible markers Cistrons The number of cistrons per marker is significant for complementation experiments and conjugation experiments that are trying to determine the number of cistrons or looking for recombination between them Beads A bead is the smallest unit of a bacterial chromosome that uGCK models roughly equivalent to 100 codons Distribution This roughly controls how many markers will be auxotrophic markers and how many resistant Degradative markers are not yet implemented they should be left at 0 Conjugation Model The Time of Entry conjugation model is the simple
37. enotype Worksheet To destroy a phenotype worksheet select it by clicking on its title and then choose Destroy Worksheet s from the Analysis menu Complementation Worksheets Complementation worksheets record the complementation behavior of a plate s colonies Depending on the way GCK is set up they either provide a place for you to record your observations or they are automatically filled out The title of the complementation worksheet indicates which plate the colonies come from and which marker is shown In Figure 55 the title tells us that this complementation worksheet records the complementation status of the colonies on plate 1 P1 for the penicillin marker Opening a Complementation Worksheet To open a complementation worksheet choose Complementation Worksheet from the Analysis menu If there is only one plate or if all plates are derived from one plate by replica plating the menu item will always be active If there are two or more possible plates with different colonies you will need to select a plate before choosing the menu item Reading a Complementation Worksheet Complementation worksheets record whether or not two strains will complement each other All the colonies in the plate are listed along the top and along the left side If there is a at the intersection of two strains it indicates that those strains do not complement A indicates that they do complement and a indicates that their status is not known
38. ewhere on the icon You can select tubes in icon form and dilute them plate them autoclave them or ask for their histories Microbial Genetics Construction Kit User Manual 41 Selecting a Tube Before you can do anything with a tube or set of tubes you need to select it To select a tube click on it somewhere Clicking on its title works fine A selected tube title will be shown as white on black instead of the unselected black on white see Figure 49 Taking Notes on a Tube Clicking on the notepad button E upper left corner of every tube will open a window which can be used for taking notes You can type into this notepad paste pictures from other GCK windows into it print it or copy it into a word processor to help you prepare your lab report uGCK automatically inserts the dilution factor used to create the plate when a tube is plated with automatic dilution Getting the History of a Tube It is easy to forget how you created a particular tube You can ask GCK to jog your memory by selecting a tube and choosing Tube History from the Tube menu uGCK will open a notepad window with a short description of where the tube came from If you select more than one tube you will get the histories of all selected tubes in one note Autoclaving a Tube If you no longer have any need for a tube you can autoclave it To autoclave a tube select it and choose Autoclave Tube from the Tube menu Since autoclaving is not reversible you w
39. f as power failure or an problem with the program that causes it to stop working suddenly When you choose Save the first time you will be asked to give the problem a name see Figure 61 If the process of giving a file a name is unfamiliar to you please refer to BioQUEST Macintosh Basics O AppleLink EEEE G Guang pagg O Communications O Deep Storage O Drawings Figure 61 A Save Problem dialog box By default the problem will be saved under the name Untitled0 When you are ready click the Save button to save the problem or click the Cancel button if you decide not to save The second time you choose Save your problem will automatically be re saved under the same name you used the first time If you want two different copies use the Save As option instead of Save This will ask you for another name Opening a Saved Problem There are two ways to open a previously saved problem The simplest way is to double click on the saved problem s icon from the Finder see Figure 62 58 Microbial Genetics Construction Kit User Manual Figure 62 A saved problem icon Alternatively if you are already running GCK you can choose Open from the File menu and choose your problem from the list presented there Note that you can only have one problem open at a time If you try to open a second problem you will first be asked if you want to save the current problem Designing Your Own Problems In order to create or
40. icillin 2 2 2 2 2 2 2 2 2 2 2 2 2 2 Rifamycid 2 72 2 2 2 72 2l2 2 l 2 72 l a e CC Figure 21 A phenotype worksheet This one has been resized to show all nutrients and all colonies 20 Microbial Genetics Construction Kit User Manual Using the phenotype worksheet is somewhat similar to using the media matrix you have already seen Nutrients and antibiotics are listed down the left side and the colonies on the field plate are listed along the top At the intersection of each nutrient row with each colony column is a cell where the relationship between the two can be recorded A question mark indicates that the relationship is unknown Click ona cell to cycle through its possible states In this example we want to record that colony A4 is an alanine prototroph and B3 and B5 are alanine auxotrophs Auxotrophy is conventionally shown with a minus sign and prototrophy is shown by a plus sign so these are the possible states of the nutrient cells of a phenotype worksheet Figure 22 shows the phenotype worksheet with the indicated information recorded This information is recorded by clicking once on the alanine A4 cell to make it a plus sign and clicking twice on the alanine B3 and alanine B5 cells to change them to minus signs This will not work in this example because this worksheet has been locked to prevent accidental changes You can unlock a worksheet by clicking on the padlock button i in the upper left
41. ill be asked for confirmation Constructing Media Several operations in GCK require you to construct a medium You construct media with the help of the media matrix shown in Figure 51 42 Microbial Genetics Construction Kit User Manual Choose Medium Ra E cancer Alanine Turdsina Tyrosine Biotin Nutrients Thiamine _ en Riboflavin Mecin l Rifamyci Nutrients Antibiotics Figure 51 Choosing the medium for a new plate Ke al fh The media matrix has a column for every existing plate and tube and a column for the new plate or tube that you are about to the create The new column is to the left of all the other media columns and immediately to the right of the list of nutrients and antibiotics In Figure 51 the new column is labeled Plate 2 because the new media will be used to create plate 2 To create the new medium fill in the blank column with the nutrients or antibiotics you want by any of the methods described below Click on a Cell To include an ingredient in the new medium click on the blank cell next to the ingredient name An ingredient is included when its cell is filled with gray To remove an ingredient click on the filled cell and it will go blank After you have clicked on a cell you can drag up or down to change other cells in the same way All Nutrients Click on this button to include all nutritional ingredients in the new medium Invert Nutrients Click on this butto
42. ing on or off An X in the box means it is turned on no X means it is turned off Click in the box to toggle between the two states ex A Choice A section of a chromosome that codes for a particular polypeptide In GCK this polypeptide is always a single step in a biosynthetic pathway Sexual reproduction in bacteria GCK conjugation is modeled on that of E Coli F plasmid mediated One bacterium the donor hfr transfers all or part of its genetic material some of which may be incorporated into the recipient F bacterium A contiguous group of isogenic bacteria derived from a single ancestor and growing on a petri plate If two mutants complement each other they are able in conjunction to express the wild phenotype The clipboard is an invisible place where something usually a picture or a few words can be stored fora moment When you Copy text you put it on the clipboard When you Paste you are pulling something off the clipboard to insert into a document The clipboard is part of the computer not part of the particular program you are using so you can use it to transfer information from one program to another Complementation that occurs between bacteria via the diffusion of pathway intermediate products between the cells Customize Dialog Box Field Population pGCK Isogenic Lawn Menu Mouse Notepad Object Phenotype Prototroph 68 Microbial Genetics Construction Kit User Manual
43. into it select parts of it to cut or copy into the clipboard and print it If you are not familiar with standard Macintosh word processing methods you should consult your Macintosh Owner s Guide for a description Microbial Genetics Construction Kit User Manual 51 Printing Notepads To print a notepad make sure that it is the frontmost window clicking somewhere in the window will make it frontmost The frontmost window is the only window which has a set of parallel horizontal lines around its title Then choose Print Notepad from the Edit menu For more information on notepad use see the section on Communicating With Other Programs Cleaning Up the Benchtop After you have been working for a while your lab bench the computer screen is likely to get quite messy The Clean Up option on the Utilities menu will straighten things up by putting things in their original places and closing certain windows Changing the Cleanup Process The standard Clean Up process places plates tubes worksheets and other windows on your screen in a way appropriate for the standard Macintosh 9 inch screen If you have a larger screen or if you do not like the way clean up works you can change it To do this choose the Clean Up Options option on the Utilities menu The window shown in Figure 57 will open The check boxes at the bottom of the window allow you to specify which windows should be automatically closed or collapsed to icon form during a c
44. is means that we cannot model interference but results in a considerable simplification in the computational complexity of the problem We calculate the proportions of various recombinants in the final population by calculating for every cistron that differs between the parental types the probability that it will enter a recipient cell in the time available and the probability that it will recombine with the recipient chromosome Since we have postulated that all recombination events are independent we then find the probability of multiple recombinants by multiplying the probabilities for individual cistrons In more detail the probability that a particular donor cistron will recombine with the recipient genome is the probability that it will enter the recipient e times the probability that it will recombine The probability of recombination is influenced strongly by the length of donor chromosome on both sides of the cistron so this calculation has to be re done for each possible length of entering chromosome 66 Microbial Genetics Construction Kit User Manual Definitions limit Maximum length of chromosome that could possibly enter the recipient This is a function of the time before agitation and the rate of chromosome transfer start length of chromosome between the transfer origin and the beginning of the entering cistron b probability of breakage between two entering chromosome beads c probability of a crossover between
45. is might be your problem You should also be able to find a document called GCK Version History This might be able to tell you something about the differences between your copy of the program and your copy of the manual Otherwise contact the person you got the program from and ask what has changed Microbial Genetics Construction Kit User Manual 71 Maybe it s a bug If the problem is not covered under the preceding topics you may have discovered a problem in the manual or in the software In either case we would like to know about it Please convey the circumstances and problem back to us Hardware and Software Requirements uGCK requires a Mac Plus or later Macintosh computer running System 6 0 or later To tell what system you are running choose the About the Finder item from the menu of the Finder program The Finder program is where you start out before you run a program like pGCK Index 57 All Nutrients 18 44 Antibiotic 49 Auto Dilution 45 Autoclave Plate 41 Tube 43 Auxotroph 49 71 Bead 63 71 Benchtop 53 Biochemical Pathway 47 Check Box 71 Choosing Media 43 Chromosome Length 63 Cistron 47 63 71 Clean up 12 53 Clean up Options 53 Clear 54 Clear Antibiotics 18 45 Clear Nutrients 18 44 Clipboard 54 72 Colonies Number of 62 Colony 71 Phenotype 48 Phenotypes 24 Selecting 27 Command Key 56 57 Complement 47 71 Complementation 27 Complementation Groups 31 Complementation Worksheet 29 50 65 C
46. l we mean something that can be selected Colonies plates tubes and worksheets are the objects in GCK The observable properties of an organism A result of the collective action of its genotype and its environment Opposite of an auxotroph A microorganism that does not require a particular nutrient for growth Microbial Genetics Construction Kit User Manual 69 Scrapbook Turbid Window The scrapbook is a desk accessory that will store more than one thing for you This is an advantage over the clipboard which can only store one thing at a time See your Macintosh Owner s Guide for more information on desk accessories and the scrapbook A tube containing so many bacteria that it visibly scatters light The opposite of a clear tube which does not have enough bacteria for the liquid medium to be unclear A window is an area of the computer screen usually rectangular that displays information Most windows have a title displayed at the top For more information see your Macintosh Owner s Guide Plates Notepads Phenotype Worksheets etc are all examples of windows 70 Microbial Genetics Construction Kit User Manual Appendices It Doesn t Work The program won t run Have you booted your system properly If this question doesn t mean anything to you please look at BioQUEST Macintosh Fundamentals or ask someone who has used a Macintosh computer before Are you using System 6 0 or later uUGCK requires system soft
47. l chromosome starting at a particular origin and in the same direction If we look at just one mating pair the chromosome is transferred from the Hfr donor to the F recipient at a roughly constant rate after a variable set up time until the connection is broken either by deliberate shaking by the experimenter or at random with a constant probability per unit time Once a segment of donor chromosome has entered the recipient cell it may recombine with the local chromosome The actual recombination process is not well understood Parts of the donor chromosome that do not recombine may persist for a while possibly even long enough to recombine with the recipient s descendants but eventually degrade Usually of course one is not dealing with a single conjugating pair but with a very large population of bacteria which meet and begin to conjugate over some time interval In this model we have made a number of simplifying assumptions First once the donor chromosome has done whatever recombining it is going to do with the initial recipient it disappears Also we assume that all pairs begin to conjugate at the same time and that chromosome transfer always occurs at the same rate roughly that of E Coli at 37 C on optimal media Then since recombination mapping using conjugation is not that common we have made the drastic assumption that the probability of a crossover between any two beads is constant independent of other nearby crossovers Th
48. late menu you will see something that looks like Figure 13 You can see that all items on the menu are gray to indicate that they are inactive If you try to select an inactive menu item in GCK it will tell you why the menu item is inactive To try this release the mouse button when it is over the Replicate item and you will see something like Figure 14 To see the remaining text move the mouse pointer over the downward pointing arrow and click To dismiss the help message click on the Cancel button Microbial Genetics Construction Kit User Manual 15 Plate Replicate In order to use this option you must first select 4 petri dish Select 4 dish by clicking ina spot where there is no colony If there are no petri dishes on the Cancel Figure 14 A help message explaining why the Replicate menu item is inactive Select a Plate This message tells you that you must select a plate before you can replicate it To do so click somewhere on the plate other than where there is a colony or a button Clicking on the plate s title works well A selected plate s title is printed in white on black instead of the normal black on white Figure 15 shows a selected plate Field Plate ENERET Figure A selected plate Note that the title is highlighted in black to indicate selection Once you have a selected a plate you can choose the Replicate item from the Plate menu Select a Medium Now you have to decide what medium you want t
49. lean up operation The box in the upper part of the window shows where each of the different kinds of windows created by GCK will be placed when it is first created and when you ask for aclean up In Figure 57 the three black plate outlines represent the placement of the first three plates later plates will be placed on top of the first three offset a little You can change the number of rows and columns of plates and the spacing between them by adjusting the large rectangle with the little grow box in the lower right corner You can change the placement of the group of all plates by dragging the big rectangle around the screen To change the placement of other kinds of windows click on the Next button to bring the next set of windows to the top or click directly on the gray boxes representing the window you want to change 52 Microbial Genetics Construction Kit User Manual Edit Bench Top Layout o H dadada aih A ahi oe T ee T s Petri Dishes Before Cleanup Collapse all petri dishes lt Collapse all test tubes lt Collapse all work sheets J Close all notes Figure 57 The Clean Up Options window Communicating With Other Programs All communication between pGCK and other programs takes place via the Macintosh Clipboard Think of the clipboard as a place you can temporarily store a piece of text or a picture from one program and then retrieve it from another program You proceed by Copying
50. lelelelelelet te Phebe lelal LLL Figure 33 An alanine complementation worksheet After you have recorded complementation information in the worksheet you may want to lock it to guard against accidental changes To lock a worksheet click on the padlock button i in the upper left corner of the window Clicking a second time will release the lock As with the phenotype worksheet you can drag rows and columns of the complementation worksheet to present the information more conveniently This can be helpful to clarify complementation groups Quitting This is the end of the tour of Complementation Testing If you want to quit at this point you can do so by choosing the Quit item from the File menu You will be asked if you want to save your work If you decide not to quit after all click on the Cancel button If you save your work the section in the reference section entitled Opening a Saved Problem will tell you how to restore the problem to where you left it If you want more detail on using plates and worksheets read the relevant sections of the Reference section If you want a taste of some of the other things that GCK can do read the other Tour sections If you want details on exactly how the computer simulates various aspects of cross feeding and inoculation read the How pGCK Works section Microbial Genetics Construction Kit User Manual 31 A Tour of Conjugation Mapping with GCK This tour assumes that you have comp
51. leted at least one of the other tours and feel comfortable with the basic mechanics of manipulating plates tubes and worksheets If you just finished a different tour you can choose New Problem from the File menu to start anew problem This is equivalent to starting the program over again Looking at Colony Phenotypes Open the phenotype worksheet by choosing the Phenotype Worksheet from the Analysis menu Notice that all the colony phenotype information has been filled in and that there is an additional row at the top of the worksheet that you have not seen before see figure 34 This row records the status of the F Plasmid in each colony Hf is an abbreviation for Hfr and refers to bacteria with the F Plasmid integrated into their chromosomes These are colonies of donor bacteria F bacteria lack the F Plasmid and are recipients during conjugation P1 Phenotypes e VOSA NNER RNS ER RDO esane ddl de fathadhatta tae EE EEE Alanine Tyrosine ar EAR hiamine l l l l l lelelele Riboflaving jacin Penicillin s s s s s s s s s s s s s s s_ Figure 34 A phenotype worksheet with F Plasmid information Columns have been rearranged to cluster Hfr and F colonies Selecting Colonies to Conjugate For this example we will conjugate bacteria from colonies A2 and D2 A2 is an Hfr colony of
52. n to reverse the status of all nutritional ingredients Clear Nutrients Click on this button to remove all nutritional ingredients from the new medium Clear Antibiotics Click on this button to remove all antibiotics from the new medium Copy Medium To copy the medium used for another plate or tube click on any of the cells for that medium The medium will be copied over into the first column Microbial Genetics Construction Kit User Manual 43 Drag Rows You can rearrange the standard order of ingredients by dragging the ingredient names up or down This will change the standard order used everywhere else as well Drag Columns You can rearrange medium columns by dragging their names around You cannot drag the first column or drag any other column into the first position Experiments with Plates Replica Plating a Plate To create a replica plate select the plate you want to replicate and choose Replicate from the Plate menu You will then need to construct a medium for the new plate as described in the section Constructing Media Experiments With Tubes Diluting a Tube To dilute a tube select it and then choose Dilute 10 Fold from the Tube menu This instructs GCK to take one milliliter of liquid from the selected tube and place it in a new tube along with 9 milliliters of distilled water You may repeat this process as many times as you think necessary to create a rack of serial dilutions After diluting a tube GCK will
53. ndows MS DOS and Windows NT are either registered trademarks or trademarks of Microsoft Corporation Helvetica Times and Palatino are registered trademarks of Linotype Hell The BioQUEST Library and BioQUEST Curriculum Consortium are trademarks of Beloit College Each BioQUEST module is a trademark of its respective institutions authors All other company and product names are trademarks or registered trademarks of their respective owners Portions of some modules software were created using Extender GrafPak by Invention Software Corporation Some modules software use the BioQUEST Toolkit licensed from Project BioQUEST TABLE OF CONTENTS What is Microbial Genetics Construction Kit ccc ecseeeeeeseeesesseesssesseseeeeeees 1 WD TOT TOCAR a terete E A erect rere 2 WY A NCO NO N aer e GE N ERE E NE TEE EEN 3 A Word ol VV ARTIS sioi eken keron Eaa r e ER Tni EN a 4 ASTIN SE ATU o E E eae ater E E E E some atenvecsmte cones 5 otlarin the POR PAI iser enr aonaran ES Ea er EENE ONEEN ERINN 5 COC Si a TOE e E sc ree otros mesnneanents 5 A Tour of Serial Dilution with GCK cccccesccesssecceseceseeeceesneceesaeeceeeeeeeneesesaees 7 The Tiela I UDE penipeni meee E A EEEE EE EAEE 7 Parna a OS a E E E EE E E E 8 TS eases spe E E 8 eee LG all OC eiii E EE E E l Plate the Tube Oni Tube MC a ssssacassnsasscwunssusasisosvnssnannantavoneseensiusswesannen 9 IB ADeby aba year tal he ol en a reer E cee cer reer E er rrerre N 10 Oo bhai
54. o be used for the new plate GCK will display a Media Matrix that allows you to specify what you want on the new plate Figure 16 is an example of such a media matrix 16 Microbial Genetics Construction Kit User Manual Choose Medium Ra E cancer Alanine T Twe Tyrosine Biotin Nutrients Thiamine Riboflaving ten Baen Rifamycit Nutrients z Antibiotics Gat Figure 16 A choose medium media matrix for replica plating This media matrix shows you the media used in all previous plates and test tubes and allows you to choose the ingredients for your new medium In the example shown here there has been only one previous plate the field plate Its medium has all nutrients and no antibiotics This is shown in the second column of the matrix by the filled cells in each of the nutrient rows and the empty cells in the antibiotic rows the two bottom rows The name at the top of the first row in the matrix Plate 2 is the name of the new plate and the column under it shows its medium Initially the medium has no nutrients and no antibiotics You can add nutrients or antibiotics by clicking in the corresponding cells The mouse arrow in figure 16 is over the cell corresponding to the nutrient alanine clicking here would add alanine to the medium for plate 2 Microbial Genetics Construction Kit User Manual 17 _ Choose Medium All Nutrients nutrients ean f Rifamycig Nutrients
55. o distinct colonies is called a lawn plate Diluting a Tube In order to have countable colonies on a plate after we plate a tube we need to lower the concentration of bacteria in the tube before plating We do this by repeatedly diluting the tube until we get discrete colonies when we plate To dilute a tube select it and choose the Dilute 10 Fold option from the Tube menu This removes one tenth of the liquid in the selected tube and adds it to a new tube nine tenths full of sterile water The result is that the population of bacteria in the second tube is one tenth as dense as it was in the first tube Notice that the diluted tube is not turbid gray indicating its lower population density Figure 8 shows the tube resulting from one dilution of the field tube Its relative population density is indicated at the bottom by the 1 It is automatically selected for you so that you can easily dilute it further or plate it to see if the population is sparse enough yet Figure 8 A ten fold dilution of the field tube Microbial Genetics Construction Kit User Manual 11 Counting Colonies Jo 12345 6 Figure 9 Plate from a tube with a million fold dilution Figure 9 is a plate produced from a tube that was diluted 6 times for a population density a million times lower than that of the original field tube remember that your bacterial population will be different Plating this tube lowered the number of bacteria by another factor of
56. o read you can draw all the grid lines by clicking on the grid button which is the set of cross hatched lines in the upper right hand corner of the window In Figure 25 the mouse arrow is shown over the grid button Microbial Genetics Construction Kit User Manual 23 Field Plate loa 23456 Figure 25 gridded plate The mouse arrow is over the grid button Figure 25 shows a plate after the grid has been turned on To turn the grid back off click on the grid button again Looking at Colony Phenotypes If you went through the previous tour Phenotype Identification you have experience determining the phenotypes of colonies and recording them in a phenotype worksheet In this tour we are going to look at complementation effects that require that we already know the phenotypes of colonies The problem used in this tour has been set up so that this work has already been done and the phenotype worksheet already filled in To open the phenotype worksheet pull down the Analysis menu and choose Phenotype Worksheet see Figure 26 PI Phenotypes Alanine ajeje ay 4 f2 thiamine LLELLE Riboflavind Penicillin s s s s s sis s sis s s s s s s s s s Ritamycitr r r r s sir sjs sjslrjslrirlsirlsisz a Figure 26 The complete phenotype worksheet for the field plate 24 Microbial Genetics Construction Kit User Manual Remember that your phenotype worksheet won t look i
57. odons and assume that this corresponds to 3 5 beads then a bead can be thought of as roughly 100 codons This means that the total range of cistron sizes available is from 100 to 1600 codons Bacterial chromosomes are often measured in minutes where a minute is the length of chromosome transferred between two conjugating bacteria at 37 C in one minute Conjugation in E Coli occurs at about 1000 base pairs per second which means that we have about 200 beads per bacterial minute Cistrons are parts of groups which together form and regulate a biochemical pathway with in this model anyway phenotypically observable results For the purposes of this model these groups of cistrons are referred to as markers A marker may consist of from one to n cistrons where n is some maximum that must be set when pGCK is compiled at the moment n 5 For now the cistrons comprising two different markers must be disjoint We would like to remove this constraint sometime Markers in GCK may be of three types Resistance Auxotrophic or Degradative Resistance markers control sensitivity and resistance to antibiotics or possibly to other chemical or phage attack Auxotrophic markers control a bacterium s ability to synthesize needed nutrients from the basic materials available in a minimal medium Degradative markers not completely implemented yet control the ability to degrade complex sugars into basic glucose The relationship between a marker and its c
58. of recombination frequencies is quite time consuming we have provided one model of conjugation which does no calculation of recombination at all It simply finds the probability of entry for markers and assumes that any marker that enters a recipient cell will be incorporated into its gnome Another model does calculate recombination probabilities but with a relatively large step size so that its accuracy over short distance is not to be trusted too far Microbial Genetics Construction Kit User Manual 67 Active Menu Active Window Auxotroph Bead Check Box Cistron Conjugate Colony Complement Clipboard Cross Feed Glossary An active menu appears as black on white This is a sign that at least one of the items on the menu is active An active menu item is one that you are currently allowed to choose Inactive menu items which appear in gray are not allowed at the moment To find out why an inactive menu item is inactive try to choose it You will get a short explanation of how to activate it The active window also called the frontmost window is the window with the horizontal lines around the title There should only be one active window See also Selected Window A microorganism that requires a nutritional supplement for growth usually because of a defect in a synthetic pathway In GCK the minimal unit of chromosomal simulation At the moment a bead is about 100 codons long A standard way to turn someth
59. omponent cistrons is extremely simple at the moment Each cistron is assumed to code for a product which takes part in a serial biochemical pathway If any part of the pathway is blocked by a defective cistron the marker is defective Each cistron product may be marked as non diffusible which means that it cannot complement at all diffusible so that it can complement another defective cistron within the same cell in a merozygote or cell wall diffusible so that two different cells can complement in a cross feeding experiment In the current GCK all cistron products are cell wall diffusible Microbial Genetics Construction Kit User Manual 65 Conjugation The model of conjugation employed by GCK is restricted to those forms of conjugation mediated by the F plasmid in the Hfr configuration At the moment there is only one insertion point for the F plasmid Once the user chooses to conjugate two populations of bacteria one of which is Hfr and one of which is F the model must model the actual act of conjugation The outcome of a conjugation cross is always described in terms of the number of resultant recombinants observable by conventional selective techniques This is used to generate initial gross maps of a genome via time of entry mapping and may also be used to some extent for more fine structure mapping by looking at recombination frequencies An isogenic Hfr strain has one particular F insertion point so it always transfers the bacteria
60. omputer Memory 47 Conjugate 47 71 Conjugation 32 Conjugation Model 64 Conjugation Time 33 Copy 54 Copy Window 55 Copy Window Data 55 Copying Media 45 Create Problem 60 Cross Feed 47 72 Cross Feeding 27 Customize 72 Cut 54 Data 55 Database 55 Delete Problem 60 Design Problem 60 Destroy Plate 41 Tube 43 Worksheet 50 Dialog Box 72 Diluting a Tube 10 Edit Problem 60 F Plasmid 32 62 65 Factor 44 Field Plate 14 23 Field Population 72 Parameters 62 Field Tube 7 Fill Complementation Worksheet 52 Fill Phenotype Worksheet 50 Frontmost Window 53 55 56 71 Graphing Program 55 Help 56 Help Mode 57 History Plate 19 Icon Plate 39 Tube 42 Worksheet 22 50 Icons Plate 12 Tube 12 Ingredient 44 Inoculate Tube 46 Inoculate Tube in New Media 27 Invert Nutrients 18 44 Isogenic 72 Lawn 72 Layout 53 Length of Chromosome 63 Macintosh 2 3 Make Problem 60 Marker Distribution 64 Markers 63 Media Choosing 43 Compare 47 Look up 47 Media Matrix 16 19 28 43 47 Medium Choosing 16 Copying 45 Memory 47 Menu Active 71 Gray 56 Help 57 Menus Changing 65 66 Mess 53 New Problem 14 Notepad 52 72 Printing 53 Nutrient 44 Choosing 29 Synthesis 49 Open Problem 60 Option Key 57 Parameters Checking 64 Field Population 62 Menu 65 66 Paste 54 Pathway 47 Phenotype 73 Phenotype Worksheet 20 24 48 65 Plate Autoclave 41 Blank 38 Destroy 41 Field 14 23 62 Grid 38 History 19 41 Icon 39
61. on from the Tube menu Choose Medium Nutrients Invert an DON BNI RDS Penicillir Rifamycit Nutrients Antibiotics Figure 38 Setting up a restrictive medium to plate the conjugant population 34 Microbial Genetics Construction Kit User Manual In this case a plating medium that is lacking in both alanine and tyrosine has been set up so that neither of the parental strains will grow but any recipient that have picked up the ala from the donor strain will grow Figure 39 shows the resulting plate Plate Figure 39 The plated result of the conjugation experiment Colonies did grow on plate 2 so we got some recombinants after 50 minutes The alanine locus is within the first 50 minutes If you want to look at the phenotypes of the colonies on this new plate you would expect to be able to ask for the phenotype worksheet If you look at the Analysis menu however you will see that the Phenotype Worksheet option is gray to indicate that it is not available This is because there are now two plates with different colonies on them and pGCK does not know which to use In this situation you must select a plate before asking for the phenotype worksheet Quitting This is the end of the tour of Conjugation If you want to quit at this point you can do so by choosing the Quit item from the File menu You will be asked if you want to save your work If you decide not to quit after all click on the Cancel button If you
62. pen a notepad window with a short description of where the plate came from If you select more than one plate you will get the histories of all selected plates in one note Autoclaving a Plate If you no longer have any need for a plate you can autoclave it To autoclave a plate select it and choose Autoclave Plate from the Plate menu Since autoclaving is not reversible you will be asked for confirmation Tubes Close Dilution Factor Figure 48 A turbid tube The blank dilution factor indicates that this tube has not been diluted Reading a Tube 40 Microbial Genetics Construction Kit User Manual Tubes are either clear or turbid The tube pictured in Figure 48 is filled with a gray pattern to show that it is turbid A turbid tube contains enough living bacteria so that the liquid is not clear A clear tube may contain living bacteria but not enough to affect the transparency of the liquid medium Figure 49 shows a clear tube Figure 49 A selected clear tube The dilution factor is one tenth Shrinking a Tube When you have several tubes on the screen you may want to shrink some of them to clear space You can do this by clicking in the close box which is the white rectangle in the upper left hand corner of the window This will cause the tube to shrink down to an icon like that shown in Figure 50 Tube 2 Figure 50 A tube that has been reduced to an icon To re expand a tube that has been shrunk double click som
63. plates in icon form and replicate them autoclave them or ask for their histories You cannot however select individual colonies Zooming a Plate You can expand a plate to a large size see Figure 46 by zooming it To zoom a plate click in its zoom box the concentric squares in the upper right To return a zoomed plate to its former size click on the zoom box again 38 Microbial Genetics Construction Kit User Manual Field Plate Figure 46 A Zoomed plate Selecting a Plate Before you can do anything with a plate or a set of plates you need to select it To select a plate click on it somewhere other than on a colony or a button Clicking on its title works fine A selected plate title will be shown as white on black instead of the unselected black on white see Figure 47 Totes 456 Figure A selected plate Note that the title Field Plate is highlighted Microbial Genetics Construction Kit User Manual 39 Taking Notes on a Plate Clicking on the notepad button E upper left corner of every plate will open a window which can be used for taking notes You can type into this notepad paste pictures from other GCK windows into it print it or copy it into a word processor to help you prepare your lab report Getting the History of a Plate It is easy to forget how you created a particular plate You can ask GCK to jog your memory by selecting a plate and choosing Plate History from the Plate menu uGCK will o
64. rent genes within a bacterium These are cases in which bacteria growing alone cannot synthesize a nutrient because of a defect in the biochemical pathway but when two or more bacteria grow together they can supply each other with necessary intermediates in the pathway and together can synthesize the nutrient This variety of complementation is called cross feeding 26 Microbial Genetics Construction Kit User Manual To conduct a cross feeding test in GCK inoculate a test tube with bacteria from two or more colonies If the test tube growth medium is lacking a nutrient that all the bacteria require there will be growth only if the bacteria can cross feed To select one colony click on it To select two or more colonies click on them while holding down the shift key In Figure 29 I have selected the two colonies C4 and C6 both auxotrophic for alanine Field Plate 2 Figure 29 Colonies C4 and C6 have been selected by clicking while holding the shift key Once you have selected the colonies you want to test choose the Inoculate Tube in New Medium option on the Colony menu This will give you a chance to select the medium you want in the new tube by showing you the media matrix see Figure 30 Microbial Genetics Construction Kit User Manual 27 Choose Medium revere SR Alanine _ Thiamine __ Ail Riboflaving ATT Tyrosine Ea ren p Nutrients Clear Antibiotics Figure 30 Choosing the medium for a new test t
65. select it by clicking anywhere in the body of the tube Cancel Figure 5 A message describing why Plate Tube on Tube Medium is gray The message in Figure 5 tells us that we need to select a test tube before we can plate it Microbial Genetics Construction Kit User Manual 9 Select the Tube To select the tube move the mouse pointer over the body of the tube and click A selected tube s title is highlighted in black see Figure 6 To unselect the tube click on it again For the moment however it should be selected so make sure that it looks like Figure 6 Figure 6 A selected tube Plate the Tube on Tube Media After you have selected a tube when you pull down the Tube menu the Plate Tube menu option will be black to indicate that it is active Choose this menu option and uGCK will spread the contents of the tube on a new petri dish incubate the dish to erow all the individual bacteria into colonies and then display the plate The nutritional medium used for the plate will be the same as that in the tube Plate 1 G E Figure 7 A petri dish with a bacterial lawn Figure 7 is the result of plating the field tube The gray material in the petri dish is a mass of bacteria In this case so many bacteria were placed on the plate that when they 10 Microbial Genetics Construction Kit User Manual incubated and grew the resulting colonies overlapped and no separate colonies are visible This kind of plate with n
66. ssesseseesesseseeseeserseessessersresesses 54 What s Unis Thing FOr coseson einan RE EEEN aN ER 54 What ADOUt The Bie PICU re scicsssassntsntssocssvaatsndsnienondsonesontscbsvantocvestns 56 Saving and Opening a Problem uu eee ee ceeeeeeseeeseeeeeeseeeseeeeeeeeeeees 56 DAN NST ODOT is E A rane sarepoe bine soensoe woarsouavous pencustiednntaocs 56 Opening a Saved Proble eee mnrnenr en neem eer ner ree ee nner eee 5 Designing your Owi Probles siscuscasssecsssbenneveastsnavnnsentowateuanvsnmbennsunoveavioes 58 Field Population Parameters escscsscaoscnsnsasrovacoontosenondeonsnnostedsntayeenawannncas 60 Genome COMMS UTA TON sscosicieriieeipiini een 61 Checking the Paramete Senensis anai 62 Merna T arame tO erann N R N RANER E 62 Pow GC VV Or R ra A E E T T A E AT 64 TNE PEES MOA rarere n E E E EE 64 Cona O e sao EE E E EAE E TE 65 RGSS AY E E A A E E A E 68 PD OC Ce A E A N T E 72 UDO N OK eei a E E E EEA E E REEE 72 Ihe progran WON TTUN emege ionia o 72 Have you booted your system properly eee eee 72 Are you using System 6 0 or later oo eeeeeeeeeeeee 72 Are you using a Macintosh Plus or later computer T2 Mape Sok oe oa er N E S 72 The program doesn t look like the picture in the manual 72 Maybe it is not supposed to look like the picture in the PU LALO I TE E omni svctabetsvsne ian ctbaretsvecacestaseses 12 Maybe you have the wrong manual eesseseeecerrererereres 72 DTA O
67. st and fastest It simply finds the probability of entry for a marker and assumes that any marker that enters a recipient cell will be incorporated into its genome The Recombination model calculates recombination probabilities and allocates the resulting population size accordingly It is a good deal slower than the Time of Entry model Checking the Parameters Once you have set up the problem type you want click on the Check button so that uGCK can check to make sure that it can create the problem that you asked for If something you asked for is impossible it will be changed to something possible when you click on the Check button Check does not check some things that it ought to check For example if you ask for more markers than you have nutrients and antibiotics available Check will not notice the problem 62 Microbial Genetics Construction Kit User Manual Menu Parameters Menu Subset O Serial Dilution Menu Subset Phenotype Identification Menu Subset Full Menus Custom Menu Subset g f ustarr Menu Options Tube Dilution x Default is automatic dilution Phenotype Worksheet L Fill out nutrient information automatically J Include plasmid information area J Fill out plasmid information automatically Complementation Worksheet Fill out Complementation Worksheet Figure 67 Menu Editing Menu Subset The menu subset options allow you to control what menus and menu options appear in a problem The first
68. tes and phenotype worksheets read the relevant sections of the Reference section If you want a taste of some of the other things that uGCK can do read the other Tour sections If you want details on exactly how the computer simulates various aspects of replica plating read the How GCK Works section 22 Microbial Genetics Construction Kit User Manual A Tour of Complementation Testing with GCK This is a tour of complementation testing with GCK If you just finished a different tour you can choose New Problem from the File menu to start a new problem This is equivalent to starting the program over again The Field Plate You should see a picture of a petri plate similar to that shown in Figure 24 You will have a different number of colonies in different places however so yours will not be identical to figure 24 Field Plate Totes 456 Figure 24 field plate Figure 24 shows a field plate Each of the gray circles represents one colony The idea is that the colonies shown on the plate were grown from bacteria collected from the field and are presented here for your analysis The colonies are of unknown genotype and phenotype although all bacteria within a colony share a genotype and phenotype The letters along the left side and the numbers along the bottom of the plate form a grid that is used to name the colonies The single colony in the top row for example is referred to as colony A4 To make the grid easier t
69. that contains the first selected colony Inoculate Tube in New Medium This will ask you to construct the medium to be used for the new tube Inoculate Tube in Last Medium This will create a new tube using the same medium used to create the last tube Microbial Genetics Construction Kit User Manual 45 Conjugating Two Strains To conjugate two strains of bacteria select the two colonies and choose Conjugate from the Colony menu You will be asked to specify how much time the two strains should be allowed to conjugate and a new tube will be created that contains the conjugant population For details on the model of conjugation used consult the section on conjugation in the How GCK Works section Unfortunately tubes created by conjugation tend to take up large quantities of computer memory It is a good idea to autoclave tubes used for conjugation as soon as you are finished with them If you think you might need a tube later you can save a copy of your problem on disk using Save As and then delete the tube You can open this saved problem later and resume work with the deleted tube Analyzing and Organizing Your Data Media Matrix The media matrix available on the Analysis menu displays the media used by all current plates and tubes It is useful when you need to look up the media used in a previous experiment or to compare two media AAs PS Saf A es PE A PE A a CAAA Ce CAAA Py Py Py Py Fy Py Py Py Py Py Py A Py ee Py
70. thout alanine so they are auxotrophic Checking the Medium It s easy to forget where a plate came from so GCK provides some tools to remind you of what you have done First you can ask to the history of a plate by selecting the plate and choosing Plate History from the Plate menu For Plate 2 this gives the information shown in Figure 19 Plate History Plate 2 Replica of Field Plate Figure 19 A plate history notepad Plate History tells you that plate 2 is a replica of the field plate but it does not give you any information about the medium used in plate 2 This information is available in the media matrix To open the media matrix choose Media Matrix from the Analysis menu Microbial Genetics Construction Kit User Manual 19 Media Matrix Tyrosine Biotin Niacin m Penicillin Rifamycin O El Figure 20 The media matrix displays the media used by all plates and tubes The media matrix shown in Figure 20 gives the additional information that the medium used for plate 2 was deficient in alanine Recording the Results Remembering all of these pieces of information and reporting them to others is quite a chore so GCK provides a standard way to record and present colony phenotype information in the phenotype worksheet Open a Phenotype Worksheet To open a phenotype worksheet choose the Phenotype Worksheet item from the Analysis menu Figure 21 shows a phenotype worksheet P1 Phenotypes Pen
71. two are standard menu subsets appropriate for the two applications The third option turns on every possible menu and every possible menu item The fourth option opens up another window see Figure 68 that allows you to individually turn particular menus or menu items on and off Tube Dilution If this item is checked plated tubes will be automatically diluted Fill Out Nutrient Information If this is checked the nutrient and antibiotic areas of a phenotype worksheet will be filled out correctly when the worksheet is first opened Include Plasmid Information If this is checked a line describing the status of the F plasmid will appear in every phenotype worksheet Fill Out Plasmid Information If this is checked the F plasmid status will be correctly filled out when a phenotype worksheet is first opened Fill Out Complementation Information If this is checked complementation worksheets will be correctly filled out when first opened Microbial Genetics Construction Kit User Manual 63 x Plate Menu J Replicate CJ History J Autoclave Plate J Tube Menu J Dilute Auto Dilute Plate On Tube J Plate On New x Plate On Last History EJ Autoclave J Colony Menu Inoculate In Plate Medium J Inoculate In New Medium J Inoculate In Last Medium J Conjugate bJ Data Menu J Media Matrix lt x Phen Worksheet Fill Phen Worksheet J Comp Worksheet GJ Fill Comp Worksheet x Destroy Worksheets J Utilities Menu
72. two chromosome beads e l probability that a particular length of donor chromosome will enter the recipient e 1 b 1 b l roughly O l probability of an odd number of crossovers in a chromosome segment of length beads O I Ll a c for oddx x 1 r probability that a cistron once in the recipient will yield a recombinant limit r ex Ostart OX start x Start The Model The probability that a cistron will enter a donor and produce a recombinant is e start r Hayes 2 mentions 06 as a reasonable value for b Curtiss 3 states that the correct value is 064 We use 06 200 0003 per bead We find a reasonable value for c from measures of linkage distances correlated with time of entry differences Hayes suggests that two markers separated by 5 minutes will exhibit a recombination probability of 50 Curtiss suggests a recombination rate of 20 per minute We derived a value of about 05 per bead for c We make a number of simplifications to lower the computational load to manageable proportions First we use a Poisson approximation to the binomial described above Second we evaluate entry and recombination probabilities not at every bead but at every nth bead The needs of students and teachers using the GCK conjugation model will vary We anticipate that most of the use of conjugation will be for time of entry mapping Since this does not require any analysis of recombination and since the calculation
73. ube Use the media matrix to select the medium for the new tube Tube 1 Click in the first column to turn nutrients on and off If a cell is gray the nutrient is included if white the nutrient is not included In this example I want to test these two colonies for their ability to grow without alanine so I will create a medium with all nutrients except for alanine Ido this by clicking the All Nutrients button to include all nutrients and then click on the alanine cell to turn it off When you have set up the appropriate medium for your test which will probably be different from the example click on the Inoculate button to create and inoculate the tube 28 Microbial Genetics Construction Kit User Manual Figure 31 A test tube that is not turbid In this case that means that there was no growth Test tubes with large populations of bacteria are turbid That is they scatter light In uGCK this is indicated by gray coloring Since the tube in Figure 31 is clear we know that there was no significant bacterial growth Colonies C4 and C6 did not cross feed They appear to have a common defective cistron in the alanine pathway Recording the Results Complementation experiments generate a great deal of data that must be recorded and manipulated to be useful GCK provides complementation worksheets to help you with this task To open one choose Complementation Worksheet from the Analysis menu Since complementation relationships will
74. ul For this purpose you can drag rows of the worksheet down to the bottom and then resize the worksheet so that you don t even see the uninteresting rows To drag a row click on the name of the row and drag the dotted outline of the row down to the bottom and release In Figure 27 we are about to drag the tyrosine row to the bottom Microbial Genetics Construction Kit User Manual 25 Pi Phenotypes Alanine Biotin Tmiemme Riboflavin Figure 27 The tyrosine row is about to be dragged down Note the dotted gray outline around the row Figure 28 shows the result of this procedure We have dragged tyrosine and biotin to the bottom and used the window grow box to shrink the window so that the bottom five rows are invisible P1 Phenotypes anme e e thiamine L Exes 9 SS S99 SE ES ESS SESE YY Niacin Figure 08 All the uninteresting nutrients were dragged to the bottom and the worksheet was Sd to exclude them You can also drag the columns of a worksheet by clicking on the colony names This is useful if you want to concentrate on the auxotrophs for only one nutrient drag them all to the left and shrink the window horizontally so that you needn t look at non auxotrophic colonies Testing for Cross Feeding The kind of complementation described in this tour is complementation between bacteria not complementation between diffe
75. um Maximum 20 Number of markers per cell Minimum Maximum 3 Distribution of the F plasmid Hir WF Figure 65 Field Population Parameter editing 60 Microbial Genetics Construction Kit User Manual The radio buttons on the first line govern whether the initial field population will be shown in a test tube or a plate If they are shown in a plate the strains will be roughly equally represented If they are shown in a tube the relative proportions will be randomly assigned so as to make serial dilution on to a restrictive medium more interesting The second line allows you to set the number of genetically distinct strains you want to be represented in the field population The number used will be between the minimum and maximum set here The third line governs how complex the genetic makeup of a particular strain will be by setting the number of markers allowed per cell A marker in this case is auxotrophy for nutrients or resistance for antibiotics The final parameter is the distribution of the F plasmid in the field population To set the distribution drag the black rectangle to show the distribution you want In Figure 65 it is set so that the entire population is F free Click the Check button to check that the parameters you have asked for here are compatible with parameters set elsewhere This check is not infallible Click Cancel to discard the changes you have made to this problem or OK to keep them G
76. ware 6 0 or later to run properly To check which version of the system software you are using choose About the Finder option under the menu Are you using a Macintosh Plus or later computer uGCK will not run on a Macintosh 128 or Macintosh 512 Maybe it s a bug If you answered yes to all of the preceding questions maybe you have discovered a problem in GCK Please report the problem and circumstances back to the program authors The program doesn t look like the picture in the manual Maybe it is not supposed to look like the picture in the manual uGCK can be modified to look quite different from what we have shown in the manual Read the section at the beginning of this document A Word of Warning to see if the difference might be something like this Also ask the person you got the program from if they have changed something If so they ought to be able to tell you what differences to expect Maybe you have the wrong manual uGCK is not in its final form so it changes periodically While we try to keep the manual up to date it does tend to lag a little behind the program It is also possible for the wrong version of the manual to accidentally be included with a program The current version of the program when the manual was last updated is printed at the bottom of every page You can find the current version of the program by running uGCK and choosing the About GCK option from the menu If the two version numbers do not match then th
77. x CleanUp EJ Clean Up Options J Edit Problems Figure 68 Custom menu editing dialog The menu parameter editing dialog see Figure 68 allows you to decide what menu options you feel should be available for your problems To toggle an entire menu on and off click on the check box with the menu name To toggle a menu option on and off click on the corresponding check box A menu or menu option without a check mark will not be visible when the problem is used 64 Microbial Genetics Construction Kit User Manual How GCK Works When uGCK starts a new problem it first has to read the problem parameters and use them to build a set of genetic rules that we will call the Species Model Once it has a species model it uses the model to create a field population of organisms and consults the model when deciding how the species should behave This description attempts to be an accurate overview of the internal model of genetics used by pGCK It is simplified so that the details don t obscure the overview and will certainly change as new genetic phenomena are added to GCK The Species Model uGCK models a bacterial chromosome as a string of beads where each bead corresponds to some constant number of codons The correspondence of codons to beads is set by the model s requirement for implementation reasons that a cistron consist of from 1 to 16 beads If we accept the common rough approximation that a cistron has about a 1000 base pairs or 350 c
78. z Antibiotics ql Gat Figure 17 The medium for plate 2 has no antibiotics and all nutrients except for alanine The four lower buttons on the left are shortcuts If you click on the top button All Nutrients it will fill in all the nutritional ingredients Invert Nutrients will make the nutritional medium the opposite of what it is before the button is pressed Clear Nutrients will remove all nutrients from the medium and Clear Antibiotics will remove all antibiotics These are particularly useful when there is a larger set of nutritional and antibiotic factors than in this example The medium shown for plate 2 in Figure 17 was created by clicking on All Nutrients and then clicking on the alanine square to remove alanine Plate When you have created the medium for your replica plate click on the Plate button to create the new plate The Cancel button would cancel the replica plating and no new plate would be created Figure 18 shows the original field plate next to the new replica plate 18 Microbial Genetics Construction Kit User Manual Field Plate LHE Plate 2 G jo 12345 6 Figure 18 The field plate and a replica side by side By comparing the two plates we can tell which colonies require alanine to grow alanine auxotrophs and which do not alanine prototrophs Colony A4 for example did not require alanine to grow so we know that it is prototrophic for alanine B3 and B5 on the other hand did not grow wi
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