Team:LCG-UNAM-Mexico:Journals:Nando's
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=='''Nando's lab journal'''== | =='''Nando's lab journal'''== | ||
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2) I need to obtain the essential region of P4 sid 1 by pcr | 2) I need to obtain the essential region of P4 sid 1 by pcr | ||
3) I need to check for the characterization of p4 as an iGEM plasmid. | 3) I need to check for the characterization of p4 as an iGEM plasmid. | ||
- | 4) I need to ligate the P4sid1 plasmid | + | 4) I need to ligate the P4sid1 plasmid |
to the BiteBack system and transform an E.coli C1-a strain with it. | to the BiteBack system and transform an E.coli C1-a strain with it. | ||
5) then we can start checking for transduction of our system. | 5) then we can start checking for transduction of our system. | ||
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During the months of June and July, I was in charge of obtaining the phages to work with, T3, T7, P2 and P4. In order to accomplish this, I emailed the "Phage people". They are: | During the months of June and July, I was in charge of obtaining the phages to work with, T3, T7, P2 and P4. In order to accomplish this, I emailed the "Phage people". They are: | ||
- | Dr. Richard Calendar.- Professor of Molecular Biology at UCB. He has gently handed phage p4 vir1, P2 vir1 and some strains to work with them: C-520, C-2423, C-1895 and C-331. | + | [http://mcb.berkeley.edu/index.php?option=com_mcbfaculty&name=calendarr Dr. Richard Calendar].- Professor of Molecular Biology at UCB. He has gently handed phage p4 vir1, P2 vir1 and some strains to work with them: C-520, C-2423, C-1895 and C-331. |
- | Dr. Giuseppe (Joe) Bertani from CalTech. He kindly sent C1a, C-117, C1906. | + | Dr. Giuseppe (Joe) Bertani from CalTech. He kindly sent [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]], C-117, C1906. |
- | Dr. Mario Soberón and Sabino Pacheco from Instituto de Biotecnología UNAM (Institute for Biotechnology of the National Autonomous University of Mexico) have kindly given us a phage T7 lysate. | + | [http://www.ibt.unam.mx/server/PRG.base?tipo:doc,dir:PRG.curriculum,par:mario Dr. Mario Soberón] and [http://www.ibt.unam.mx/server/PRG.base?tipo:doc,dir:PRG.curriculum,par:spacheco Sabino Pacheco] from Instituto de Biotecnología UNAM (Institute for Biotechnology of the National Autonomous University of Mexico) have kindly given us a phage T7 lysate. |
- | Dr. Ian Molineux from the University of Texas gently sent us phage T3. | + | [http://www.icmb.utexas.edu/cmb/directory/details.asp?id=1707 Dr. Ian Molineux] from the University of Texas gently sent us phage T3. |
P4 sid1.- obtained from ATCC | P4 sid1.- obtained from ATCC | ||
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I started organizing the phage titration. You start from a phage lysate as a 1:1 sample, make a dilution of 1:9 of that one for a 1/10, and repeat for the new dilutions until you reach the desired dilution: from 10^-7 to 10^-13. This way you can correlate the number of plaques formed with the dilution of the stock. For example, if you only get one plaque in a 10^-10 dilution, you can state that your lysate has 10^10 plaque forming units (pfu) in the volume unit you started with. | I started organizing the phage titration. You start from a phage lysate as a 1:1 sample, make a dilution of 1:9 of that one for a 1/10, and repeat for the new dilutions until you reach the desired dilution: from 10^-7 to 10^-13. This way you can correlate the number of plaques formed with the dilution of the stock. For example, if you only get one plaque in a 10^-10 dilution, you can state that your lysate has 10^10 plaque forming units (pfu) in the volume unit you started with. | ||
- | Today, overnight standing cultures of C1a, BL-21 were left to grow at 37 degrees in order to assay for the viability of T3 tomorrow. One of C117 was placed for storing the supernatant next day. | + | Today, overnight standing cultures of [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]], BL-21 were left to grow at 37 degrees in order to assay for the viability of T3 tomorrow. One of [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]] was placed for storing the supernatant next day. |
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After some time, the cultures were crystal clear, what qualitatively demonstrated the lysis of the culture by phage T3. | After some time, the cultures were crystal clear, what qualitatively demonstrated the lysis of the culture by phage T3. | ||
- | The C117 overnight culture was centrifuged at 13000 rpm to pellet the cells and store the supernatant. | + | The [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]] overnight culture was centrifuged at 13000 rpm to pellet the cells and store the supernatant. |
- | Today, an overnight of C 2423 and | + | Today, an overnight of C 2423 and [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] were put to grow. |
Plan for tomorrow.- prepare the plaque assay for P4 sid1. | Plan for tomorrow.- prepare the plaque assay for P4 sid1. | ||
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1.NCLB- bacteria grow.- probably due to mistake in procedure. | 1.NCLB- bacteria grow.- probably due to mistake in procedure. | ||
- | 2. | + | 2.NC[[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]].- Negative control for [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] (contamination control).- grows well without plaques |
- | 3. | + | 3.[[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]]P4sid1 1.- some small plaques really far away from each other. probably because some P2 and coinfection in the ATCC lysate |
- | 4.- | + | 4.-[[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]]P4sid1 2- some small plaques really far away from each other. probably because some P2 and coinfection in the ATCC lysate (a really curious effect) |
- | 5.-C2423 P4sid1 3- many well-defined plaques (internal control discards contamination) | + | 5.-[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] P4sid1 3- many well-defined plaques (internal control discards contamination) |
- | 6.-C2423 P4sid1 4- many well-defined plaques | + | 6.-[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] P4sid1 4- many well-defined plaques |
- | 7.-C2423 P4sid1 5- many well-defined plaques | + | 7.-[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] P4sid1 5- many well-defined plaques |
- | 8.-C2423 CN.- no plaques :D | + | 8.-[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] CN.- no plaques :D |
Conclusion of the first part of the experiment.- P4 sid1 does work in the formation of plaques. P2 is actually produced in lysis, but in a really low number. | Conclusion of the first part of the experiment.- P4 sid1 does work in the formation of plaques. P2 is actually produced in lysis, but in a really low number. | ||
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colonies | colonies | ||
- | 1, 2, 3, 4, 5, 6.- different culture zones in the C1a plate which are not plaques . theoretically, may be one of these colonies could have been infected and transduced by P4, so I must assay for the presence of plaques. However, it comes into mind how i will assess the presence ot P4 inside of these bacteria by only means of plaque assays, given that P2 is a complete phage and could perform lysis on its own. This would mean to make a comparison between lysis of P2 alone and along with P4, and it's probably non-trivial to distinguish P4 plaques from P2 plaques. given all this, We should investigate about a better way to test with an internal control. Of course, the biobrick with a color signal could be excelent as an indicator, but we cannot wait for that. | + | 1, 2, 3, 4, 5, 6.- different culture zones in the [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] plate which are not plaques . theoretically, may be one of these colonies could have been infected and transduced by P4, so I must assay for the presence of plaques. However, it comes into mind how i will assess the presence ot P4 inside of these bacteria by only means of plaque assays, given that P2 is a complete phage and could perform lysis on its own. This would mean to make a comparison between lysis of P2 alone and along with P4, and it's probably non-trivial to distinguish P4 plaques from P2 plaques. given all this, We should investigate about a better way to test with an internal control. Of course, the biobrick with a color signal could be excelent as an indicator, but we cannot wait for that. |
x,y,z.- zones of the bacterial plate generated that include plaques from P2 presence. | x,y,z.- zones of the bacterial plate generated that include plaques from P2 presence. | ||
the presence of plaques reveals an interesting phenomenon; the P4 sid1 purchased stock has some P4 contamnation because it's a lysate. Dr. Bertani argues that it is of really low significance since one P2 is produced by 100 P4. The fact that you can see plaques involves that the P2 that come out are really efficient infectors of the neighbor cells, which happen to be in a P4-filled environment. If this werent the real way, the P2 phage wold be lost in the medium and, ocasionally, a cell would die, but that wouldn't necessarily produce a plaque in the agar. | the presence of plaques reveals an interesting phenomenon; the P4 sid1 purchased stock has some P4 contamnation because it's a lysate. Dr. Bertani argues that it is of really low significance since one P2 is produced by 100 P4. The fact that you can see plaques involves that the P2 that come out are really efficient infectors of the neighbor cells, which happen to be in a P4-filled environment. If this werent the real way, the P2 phage wold be lost in the medium and, ocasionally, a cell would die, but that wouldn't necessarily produce a plaque in the agar. | ||
- | E,F,G.- C2423 zones from August 14, 09 which were picked very carefully trying not to obtain any plaques. These work as pneative controls. | + | E,F,G.- [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] zones from August 14, 09 which were picked very carefully trying not to obtain any plaques. These work as pneative controls. |
In other respects, we tried to infect bacteria in M9LB without calcium to see if that worked. The incubations were made with 100 ul of phage. Lysis didn't start, so we cannot combine the protocols for both phages and calcium is really important for P4 adsorption. I need to find out how to carry out the protocol with the materials we have here. | In other respects, we tried to infect bacteria in M9LB without calcium to see if that worked. The incubations were made with 100 ul of phage. Lysis didn't start, so we cannot combine the protocols for both phages and calcium is really important for P4 adsorption. I need to find out how to carry out the protocol with the materials we have here. | ||
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bacteria expected | bacteria expected | ||
No bacteria clear dish | No bacteria clear dish | ||
- | C1a being tested for P4 sid 1 x 2 plaques if infected with P4, no plaques if not | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] being tested for P4 sid 1 x 2 plaques if infected with P4, no plaques if not |
- | C117 small plaques | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]] small plaques |
- | C2423 large plaques | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] large plaques |
C1906 no plaques | C1906 no plaques | ||
- | =='''August 21, 2009.'''== | + | =='''August 21, 2009.'''== |
We have officially confirmed yeast contamination in the lab. Many petri plates have acquired a shiny white appearance. This is a big problem, since maybe many of the results expected before now are modified by the contamination. Undoubtedly, this will lag the development of the project. The next best option will be to produce streptomycin resistant strains of every strain present until this moment. The only thing left to be done to leave this round of experiments, since the negative results from the last experiment may be due to the lack of virulence of phage P2, is to probe the absence of P4 through colony PCR product analysis. The PCR was performed. | We have officially confirmed yeast contamination in the lab. Many petri plates have acquired a shiny white appearance. This is a big problem, since maybe many of the results expected before now are modified by the contamination. Undoubtedly, this will lag the development of the project. The next best option will be to produce streptomycin resistant strains of every strain present until this moment. The only thing left to be done to leave this round of experiments, since the negative results from the last experiment may be due to the lack of virulence of phage P2, is to probe the absence of P4 through colony PCR product analysis. The PCR was performed. | ||
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1.C1895 | 1.C1895 | ||
- | + | 2[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] | |
- | 3.C331 | + | 3.[[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] |
4.C1906 | 4.C1906 | ||
5.C520 | 5.C520 | ||
- | 6. | + | 6.[[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]]a |
- | 7. | + | 7.[[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]]b |
- | 8.C1a | + | 8.[[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] |
Almost at the end of the day, we noticed that Juan Pablo was not told by anyone to prepare the streptomycin solution, but fortunately, we found him and he gave us some sp 100 solution, assuring that it was streptomycin. So we proceeded to prepare plates for tomorrow's assay. | Almost at the end of the day, we noticed that Juan Pablo was not told by anyone to prepare the streptomycin solution, but fortunately, we found him and he gave us some sp 100 solution, assuring that it was streptomycin. So we proceeded to prepare plates for tomorrow's assay. | ||
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C 1895.- small colony spots... | C 1895.- small colony spots... | ||
- | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]].- 2 or 3 colonies. let's check for morphology | |
- | C331 nothing yet. let's wait a bit more. | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] nothing yet. let's wait a bit more. |
C1906.- really lots of colonies. maybe the antibiotic went wrong. | C1906.- really lots of colonies. maybe the antibiotic went wrong. | ||
C520.- too many colonies. check for resistance again. | C520.- too many colonies. check for resistance again. | ||
- | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]b.- let's wait for them to grow a bit more. | |
- | C1a.- nothing clear. | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]].- nothing clear. |
- | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]a.- practically nothing | |
CN.- nothing | CN.- nothing | ||
I planned to repeat the resistant-growth assay, but the cultures I left inan overday showed contamination in the negative control. | I planned to repeat the resistant-growth assay, but the cultures I left inan overday showed contamination in the negative control. | ||
- | Late at night, I offered Paz my help in purifying PCR products. I commited a really stupid mistake when using the elution buffer before the wash buffer and treating the flowthrough as waste. I was completely ashamed of my error!!! Luckily, the PCR could be done again. | + | Late at night, I offered [[Team:LCG-UNAM-Mexico/Team/Paz| Paz]] my help in purifying PCR products. I commited a really stupid mistake when using the elution buffer before the wash buffer and treating the flowthrough as waste. I was completely ashamed of my error!!! Luckily, the PCR could be done again. |
- | Laura had left some cultures she asked me to plate. | + | [[Team:LCG-UNAM-Mexico/Team/Laura| Laura]] had left some cultures she asked me to plate. |
=='''August 27, 2009'''== | =='''August 27, 2009'''== | ||
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=='''August 28, 09'''== | =='''August 28, 09'''== | ||
- | Yeserday I plated the hypothetical P4-infected C1a for resistants. the results are the following: | + | Yeserday I plated the hypothetical P4-infected [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] for resistants. the results are the following: |
Negative control.- not valid since has colonies and yeast. | Negative control.- not valid since has colonies and yeast. | ||
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All this, except box 4, state that contamination is inminent and it is not good to try a PCR with this. | All this, except box 4, state that contamination is inminent and it is not good to try a PCR with this. | ||
- | As some of the strains have not generated resistants, yesterday Laura put overnight cultures for C1895, C2423 and C520. I have plated them. | + | As some of the strains have not generated resistants, yesterday Laura put overnight cultures for C1895, [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] and C520. I have plated them. |
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C1906 sp+.- normal, somehow brown. doesn't become yellow even after a lot of time. | C1906 sp+.- normal, somehow brown. doesn't become yellow even after a lot of time. | ||
- | C117 a1 and a2.- it's becoming fatter and fatter each time and happens to overlap with another colony. | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]]] a1 and a2.- it's becoming fatter and fatter each time and happens to overlap with another colony. |
before resistance, C1906 was yellowish with a bright halo around the colony. internal appearance looks good. | before resistance, C1906 was yellowish with a bright halo around the colony. internal appearance looks good. | ||
- | the plate with C2423 didn't grow anything before and now we have some orange round colonies in the agar. Undoubtedly, this means contamination. | + | the plate with [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] didn't grow anything before and now we have some orange round colonies in the agar. Undoubtedly, this means contamination. |
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I will try to check colony 6 for infection with p4 sid1. First, I must prepare the cell extract. | I will try to check colony 6 for infection with p4 sid1. First, I must prepare the cell extract. | ||
- | =='''September 2,2009'''== | + | =='''September 2, 2009'''== |
Objective of yesterday's PCRs.- | Objective of yesterday's PCRs.- | ||
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Plans for the rest of the week.- | Plans for the rest of the week.- | ||
- | obtain sp resistant C1a | + | obtain sp resistant [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] |
- | grow log phase C1a and add P4sid1. then plate for individual colonies. | + | grow log phase [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] and add P4sid1. then plate for individual colonies. |
we have to manage to prove that our primers work. | we have to manage to prove that our primers work. | ||
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2 tubes for C1906 | 2 tubes for C1906 | ||
- | DNA C1a.- Negative control 1 | + | DNA [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]].- Negative control 1 |
No DNA | No DNA | ||
Straight PCR | Straight PCR | ||
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Todays goals: | Todays goals: | ||
Set yesterday's PCR | Set yesterday's PCR | ||
- | Plate C1a (this is the most needed strain for infecting with P4) | + | Plate [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] (this is the most needed strain for infecting with P4) |
Laura gave me the job of taking the photographs for her phage plates. unfortunately, I didn't receive full instructions about the management of the plates and didn't think that the plaques would extend much at room temperature. well, they did. She got a bit angry because we lost a pair of plates that were krystal clear. | Laura gave me the job of taking the photographs for her phage plates. unfortunately, I didn't receive full instructions about the management of the plates and didn't think that the plaques would extend much at room temperature. well, they did. She got a bit angry because we lost a pair of plates that were krystal clear. | ||
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continuing scavenge for resistants. | continuing scavenge for resistants. | ||
- | I will grow an overnight of C1906 and C2423 to prove presence of P4 and P2. | + | I will grow an overnight of C1906 and [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] to prove presence of P4 and P2. |
if we can observe a template DNA,PCR will be performed. | if we can observe a template DNA,PCR will be performed. | ||
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Let's see if we've got template for kit-purified C1906 and the strains that were extracted DNA manually. They are.- | Let's see if we've got template for kit-purified C1906 and the strains that were extracted DNA manually. They are.- | ||
- | ones are C1906 sp resistant colonies. twos are C2423 sp resistant colonies. | + | ones are C1906 sp resistant colonies. twos are [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] sp resistant colonies. |
11 | 11 | ||
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22 | 22 | ||
- | At the end of the day, we can see that there isn't a successful genomic C2423 DNA extraction, but C1906 happens to show (dirty) DNA template, so I will run a gel for this | + | At the end of the day, we can see that there isn't a successful genomic [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] DNA extraction, but C1906 happens to show (dirty) DNA template, so I will run a gel for this |
=='''September 7 2009'''== | =='''September 7 2009'''== | ||
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Next step is to repeat the PCR of C1906. Corrections will be.- dilute 1 part C1906 DNA in 10 water. | Next step is to repeat the PCR of C1906. Corrections will be.- dilute 1 part C1906 DNA in 10 water. | ||
I'll check the annealing temperature. | I'll check the annealing temperature. | ||
- | this time, were short of DNTPs and there is a stock that was made to test. Sadly, I was a victim of Paz and he gave me useless DNTPs. | + | this time, were short of DNTPs and there is a stock that was made to test. Sadly, I was a victim of [[Team:LCG-UNAM-Mexico/Team/[[Team:LCG-UNAM-Mexico/Team/Paz| Paz]] and he gave me useless DNTPs. |
=='''September 8, 2009'''== | =='''September 8, 2009'''== | ||
Plans for the day.- wait for DNTPs to perform PCR. | Plans for the day.- wait for DNTPs to perform PCR. | ||
- | Extract DNA from C1895 and C331 | + | Extract DNA from C1895 and [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] |
I'm planning the obtention of lysate from P4 sid1 this time.- | I'm planning the obtention of lysate from P4 sid1 this time.- | ||
Obtain an aliquot of P4sid 1 by diluting it in LB supplemented with calcium. | Obtain an aliquot of P4sid 1 by diluting it in LB supplemented with calcium. | ||
- | Put an overnight culture of C1895 and add phage to it. follow | + | Put an overnight culture of C1895 and add phage to it. follow [[Team:LCG-UNAM-Mexico/Resources/Protocols/P4 |growth of p4 protocol]]. |
The PCR was interrupted by careless connection of the PCR cycler to the direct current. this was around cycle 24. | The PCR was interrupted by careless connection of the PCR cycler to the direct current. this was around cycle 24. | ||
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The C 1895 used was a sp+ one which was really slow growing. | The C 1895 used was a sp+ one which was really slow growing. | ||
Two lysis experiments were made.- one flask was added 80 ul diluted lysate from ATCC and will be called Stock (S) | Two lysis experiments were made.- one flask was added 80 ul diluted lysate from ATCC and will be called Stock (S) | ||
- | the other one was carefully picked with 2 plaques from the C2423 lysis produced in a plaque assay on August 19. | + | the other one was carefully picked with 2 plaques from the [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] lysis produced in a plaque assay on August 19. |
- | Cynthia (nené)helped me understand how to use the spectrophotometer. I turned it on for my measures. | + | Cynthia (nené) helped me understand how to use the spectrophotometer. I turned it on for my measures. |
I found the spec turned off twice while I was taking my measures. | I found the spec turned off twice while I was taking my measures. | ||
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I'll use smaller flasks since the fernbach doesn't fit inside our incubator. | I'll use smaller flasks since the fernbach doesn't fit inside our incubator. | ||
The bacteria grew really slow. That means, about .01 A600 in 3 hours. My best bet will be to leave the culture overnight and see what happened in the morning. | The bacteria grew really slow. That means, about .01 A600 in 3 hours. My best bet will be to leave the culture overnight and see what happened in the morning. | ||
- | I consider the experiment failed, so I'll have to try with a wt bacterium. | + | I consider the experiment failed ([[Team:LCG-UNAM-Mexico:Journals:Nando's#September 19, 2009|check plaque assay on Sep. 19]]), so I'll have to try with a wt bacterium. |
Today I also ran a pcr with various controls and primers. | Today I also ran a pcr with various controls and primers. | ||
only with int P4 primers.- | only with int P4 primers.- | ||
- | CN | + | CN<br> |
- | C1906 colony 2- expected: 3 kb band | + | C1906 colony 2- expected: 3 kb band<br> |
- | C1906 colony 3-expected: 3 kb band | + | C1906 colony 3-expected: 3 kb band<br> |
- | C1906 non-resistant, kit purified from stock-expected:3 kb band | + | C1906 non-resistant, kit purified from stock-expected:3 kb band<br> |
--- | --- | ||
P4 int and P2 ogr primers.- | P4 int and P2 ogr primers.- | ||
- | C2423 colony 2-expected:300 bp band | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] colony 2-expected:300 bp band |
- | C2423 colony 3-expected:300 bp band | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] colony 3-expected:300 bp band |
- | C331 -expected: 3kb and 300 bp band | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] -expected: 3kb and 300 bp band |
--- | --- | ||
P2 ogr primers only | P2 ogr primers only | ||
- | C117- expected:300 bp band | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C117]]- expected:300 bp band |
C1906 non resistant-expected: nothing | C1906 non resistant-expected: nothing | ||
- | C2423 colony 2- expected-nothing | + | [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] colony 2- expected-nothing |
- | + | ||
- | + | ||
- | + | ||
+ | results.- a strange +- 6 b band appeared in [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] which twists my mind out. It is possible that I am retrieving a product specific for the primer combination used, so the PCR isn't really valid. Hypotheses are that this newly combined pair of primers | ||
=='''September 10, 2009'''== | =='''September 10, 2009'''== | ||
- | I notice a strange phenomenon in yesterday's flasks: they have some things floating. I checked the absorbance of the culture and it was just opposite in quantity from last night's measures, | + | I notice a strange phenomenon in yesterday's flasks: they have some things floating. I checked the absorbance of the culture and it was just opposite in quantity from last night's measures; in other words, one was higher than the other and now roles have changed . I added [http://en.wikipedia.org/wiki/EGTA_(chemical) EGTA] and MgCl2. An hour later, I rechecked the absorbance and it had diminished by half in both cultures. just when lysis stopped, I added more MgCl2 to stabilize the phage and stored the hypothetical lysates in the fridge. |
=='''September 15, 2009'''== | =='''September 15, 2009'''== | ||
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Today I'll learn how to prepare LB medium and will prepare 1 liter. | Today I'll learn how to prepare LB medium and will prepare 1 liter. | ||
- | September 16 09 | + | =='''September 16 09'''== |
P4 production assay (reloaded) | P4 production assay (reloaded) | ||
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Plans for tomorrow.- Assay for presence of P$ in test growth. | Plans for tomorrow.- Assay for presence of P$ in test growth. | ||
I will need more top agarose, so I'll prepare some tomorrow. | I will need more top agarose, so I'll prepare some tomorrow. | ||
- | What I'll do.- Plate C2423 on top agarose: | + | What I'll do.- Plate [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] on top agarose: |
no phage | no phage | ||
Line 417: | Line 408: | ||
Digest with proteinase K | Digest with proteinase K | ||
Perform PCR for P4 parts: int and main (sid?) | Perform PCR for P4 parts: int and main (sid?) | ||
- | perform C1a p4 sid1 infection assay and verify with PCR. | + | perform [[Team:LCG-UNAM-Mexico/Resources/Strains|C1a]] p4 sid1 infection assay and verify with PCR. |
Tomorrow.- | Tomorrow.- | ||
- | Infect C2423 wt/sp+ | + | Infect [[Team:LCG-UNAM-Mexico/Resources/Strains|[[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] wt/sp+ |
- | September 18, 2009 | + | =='''September 18, 2009'''== |
- | I will attempt to produce plaques with P4 from different sources in the same host strain.- C2423. | + | I will attempt to produce plaques with P4 from different sources in the same host strain.- [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]]. |
S- stock lysate from september 9 involving slow-growing c1895 mutant. | S- stock lysate from september 9 involving slow-growing c1895 mutant. | ||
P.- plaque lysate from september 9 | P.- plaque lysate from september 9 | ||
Line 431: | Line 422: | ||
This is to assess the best technique to produce P4 stock. | This is to assess the best technique to produce P4 stock. | ||
- | September 19, 2009 | + | =='''September 19, 2009'''== |
Fortunately, plaques were produced. herewith the results.- | Fortunately, plaques were produced. herewith the results.- | ||
Line 441: | Line 432: | ||
- | Conclusion.- It seems that the stock produced from the slow growing mutant is far better that the one produced from the sole stock. I will try producing the stock with the | + | Conclusion.- It seems that the [[Team:LCG-UNAM-Mexico:Journals:Nando's#September 9, 09| stock produced]] from the [[Team:LCG-UNAM-Mexico/Resources/Strains|slow growing mutant]] is far better that the one produced from the sole stock. I will try producing the stock with the wild-type strain before keeping and characterizing this mutation. |
My plan for today was stopped, since the culture for C1895 didn't grow at all. | My plan for today was stopped, since the culture for C1895 didn't grow at all. | ||
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possible explanations.- the bacterial colony picked was one that came from a glycerol stock. The reseed should have been picked. | possible explanations.- the bacterial colony picked was one that came from a glycerol stock. The reseed should have been picked. | ||
Another explanation could be an aeration effect. The tube wasn't covered with a cotton lid. | Another explanation could be an aeration effect. The tube wasn't covered with a cotton lid. | ||
- | + | Today's work was reduced to.- | |
+ | 1. find out how the centrifuge works. | ||
2. find out the characteristics of the rotor used in order to concentrate the phage as the calendar protocol. | 2. find out the characteristics of the rotor used in order to concentrate the phage as the calendar protocol. | ||
3. concentrate the phage in Falcon tubes with P4 buffer | 3. concentrate the phage in Falcon tubes with P4 buffer | ||
Line 458: | Line 450: | ||
After centrifugation, the tubes were drained in a paper towel and added .25 ml of P4 buffer as the protocol indicates. The pellets will be allowed to resuspend all night in the refrigerator, then centrifugated in eppendorfs to further remove cell debris. | After centrifugation, the tubes were drained in a paper towel and added .25 ml of P4 buffer as the protocol indicates. The pellets will be allowed to resuspend all night in the refrigerator, then centrifugated in eppendorfs to further remove cell debris. | ||
- | September 20, 2009 | + | =='''September 20, 2009'''== |
Plaque assays for today.- | Plaque assays for today.- | ||
Line 467: | Line 459: | ||
- | september 21, 2009 | + | =='''september 21, 2009'''== |
The first part was completed succesfully, but 1 ml extra 1mM CaCl2 was added to the overnight culture. It is important to mention that the overnight culture was incubated with two plaques. More supplemented LB medium was prepared for stock growth. | The first part was completed succesfully, but 1 ml extra 1mM CaCl2 was added to the overnight culture. It is important to mention that the overnight culture was incubated with two plaques. More supplemented LB medium was prepared for stock growth. | ||
- | September 23, 2009 | + | =='''September 23, 2009'''== |
So, having already created stock of P4, we have to manage how to extract the DNA from phage capsids. this is the next goal since we cannot amplify P$ regions from the lysogens we have. In turn we have to really control for the presence of P4 with the lack of amplification in order to discard the primers. Meanwhile, we have designed two more primers around the sid gene region. | So, having already created stock of P4, we have to manage how to extract the DNA from phage capsids. this is the next goal since we cannot amplify P$ regions from the lysogens we have. In turn we have to really control for the presence of P4 with the lack of amplification in order to discard the primers. Meanwhile, we have designed two more primers around the sid gene region. | ||
Line 476: | Line 468: | ||
the techniques involved use phenol chloroform extractions, formamide and isoamyl alcohol. It is said that phenol, the aqueous phase, is the one that stays with the DNA and Chloroform, the organic phase, stays with the proteins, although this doesn't make complete sense, because the same mix is used to isolate phage particles. | the techniques involved use phenol chloroform extractions, formamide and isoamyl alcohol. It is said that phenol, the aqueous phase, is the one that stays with the DNA and Chloroform, the organic phase, stays with the proteins, although this doesn't make complete sense, because the same mix is used to isolate phage particles. | ||
- | September 23, 2009 | + | =='''September 23, 2009'''== |
Phage assay.- | Phage assay.- | ||
Line 488: | Line 480: | ||
These tubes can now be titered. | These tubes can now be titered. | ||
- | september 24, 2009 | + | =='''september 24, 2009'''== |
Phage DNA extraction.- | Phage DNA extraction.- | ||
Line 497: | Line 489: | ||
What substance will you use to separate capsid proteins from DNA? | What substance will you use to separate capsid proteins from DNA? | ||
- | After talk with Miguel, many things used int he protocols were clarified.- | + | After talk with [[Team:LCG-UNAM-Mexico/Team/Miguel|Miguel]], many things used int he protocols were clarified.- |
glycogen.- used to condense DNA. formamide.- to further denature proteins | glycogen.- used to condense DNA. formamide.- to further denature proteins | ||
Line 503: | Line 495: | ||
and many things are lacking, like cetyl trimethyl ammonium bromide. | and many things are lacking, like cetyl trimethyl ammonium bromide. | ||
- | September 27, 2009 | + | =='''September 27, 2009'''== |
There are 2 things that are worth testing. Dr. Calendar isolates Phage P4 DNA from a Diethyl amino ethyl cellulose (DEAE) column. The most alike element is a Phage DNA extraction kit. While the protocol handed by Rosa lasts about 3 days, this kit promises DNA within 5 hours. | There are 2 things that are worth testing. Dr. Calendar isolates Phage P4 DNA from a Diethyl amino ethyl cellulose (DEAE) column. The most alike element is a Phage DNA extraction kit. While the protocol handed by Rosa lasts about 3 days, this kit promises DNA within 5 hours. | ||
The other one is a protocol that Dr. Kameyama from Cinvestav uses. Hopefully he will send it to us soon. | The other one is a protocol that Dr. Kameyama from Cinvestav uses. Hopefully he will send it to us soon. | ||
We have to manage to get funding for the purchase of such kit by now. | We have to manage to get funding for the purchase of such kit by now. | ||
- | September 28, 2009 | + | |
+ | =='''September 28, 2009'''== | ||
We need to exchange at least one of the TOPO XL cloning kits we bought in advance. Dr. Pablo Vinuesa has to check whether he needs the TOPO cloning kit or not. | We need to exchange at least one of the TOPO XL cloning kits we bought in advance. Dr. Pablo Vinuesa has to check whether he needs the TOPO cloning kit or not. | ||
- | September 29, 2009 | + | =='''September 29, 2009'''== |
I have found another alternative: to apply the DNA extraction method from T7. it involves usage of ethanol , EDTA and heat. | I have found another alternative: to apply the DNA extraction method from T7. it involves usage of ethanol , EDTA and heat. | ||
- | I commited a small mistake in which i may have mistaken the correct phage-containing tube | + | I commited a small mistake in which i may have mistaken the correct phage-containing tube. |
- | No pellet is seen at the bottom of the tube after addition of ethanol and centrifugation. This is suspitious | + | No pellet is seen at the bottom of the tube after addition of ethanol and centrifugation. This is suspitious. |
- | September 30, 2009 | + | =='''September 30, 2009'''== |
The DNA heat burst and ethanol precipitation failed. the suspects are the following: | The DNA heat burst and ethanol precipitation failed. the suspects are the following: | ||
- | |||
No DNA was extracted from the capsids (The phage are still viable) | No DNA was extracted from the capsids (The phage are still viable) | ||
- | The phages didn't burst.- we need a better denaturing agent, like urea. This could be due to extreme phage capsid stability. | + | The phages didn't burst.- we need a better denaturing agent, like [http://en.wikipedia.org/wiki/Urea urea]. This could be due to extreme phage capsid stability. |
- | DNAse somehow managed to destroy the DNA when it was just liberated from the capsid. | + | [http://en.wikipedia.org/wiki/Deoxyribonuclease_I DNAse I] somehow managed to destroy the DNA when it was just liberated from the capsid. |
Tomorrow.- produce more P4 stock. | Tomorrow.- produce more P4 stock. | ||
- | October 2 to 4, 2009 | + | =='''October 2 to 4, 2009'''== |
Several attempts to produce Phage P4 stock have been tried. Something strange is happening. lysis won't continue after it starts and I add EGTA and MgCl2. We suspect that P4 sid1 virulence is even more dependent on calcium in the medium, so for the next attempts, I won't add the chelator at lysis start. | Several attempts to produce Phage P4 stock have been tried. Something strange is happening. lysis won't continue after it starts and I add EGTA and MgCl2. We suspect that P4 sid1 virulence is even more dependent on calcium in the medium, so for the next attempts, I won't add the chelator at lysis start. | ||
- | october 5, 2009 | + | =='''october 5, 2009'''== |
Line 548: | Line 540: | ||
- | I poured fractions of | + | I poured fractions of Friday's lysate flask 1 and 2 and named them as follows.- |
oct 2 1.1 | oct 2 1.1 | ||
Line 557: | Line 549: | ||
I also used two tubes from september 30's lysate which I wasn't able to centrifugate due to rotor space. the main idea of centrifugating is to clear out the cell debris from the lysate | I also used two tubes from september 30's lysate which I wasn't able to centrifugate due to rotor space. the main idea of centrifugating is to clear out the cell debris from the lysate | ||
- | and to further process the lysate until concentrating the phage or using it as the kit starting material. First I have to test for the presence of phage, so I will spend today concentrating the phage completely and testing for the infection of C2423, the indicator strand, in plaque production before and after concentrating the phage. | + | and to further process the lysate until concentrating the phage or using it as the kit starting material. First I have to test for the presence of phage, so I will spend today concentrating the phage completely and testing for the infection of [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]], the indicator strand, in plaque production before and after concentrating the phage. |
I also started a protocol to produce more lysate, this time without adding the EGTA, so the calcium is not chelated too soon. I verified lysis start in two flasks previously added bacteria incubated with phage about 2 hours after growth start. one of the flasks started lysing at A600 .66 and the other one at .4. | I also started a protocol to produce more lysate, this time without adding the EGTA, so the calcium is not chelated too soon. I verified lysis start in two flasks previously added bacteria incubated with phage about 2 hours after growth start. one of the flasks started lysing at A600 .66 and the other one at .4. | ||
- | October 6, 2009 | + | =='''October 6, 2009'''== |
We had an iGEM meeting where we discussed about some aspects of the presentation, wiki, poster and other stuff. I checked the A600 of the cultures I left last night and it wass about 0.65 in both, so lysis stopped at some point and the bacteria continued growing. | We had an iGEM meeting where we discussed about some aspects of the presentation, wiki, poster and other stuff. I checked the A600 of the cultures I left last night and it wass about 0.65 in both, so lysis stopped at some point and the bacteria continued growing. | ||
- | I'm really excited because the lambda DNA purification kit just arrived around 4 pm! so I'll get my DNA today and start with PCRs tomorrow (or maybe today). | + | I'm really excited because the lambda DNA purification kit just arrived around 4 pm! so I'll get my DNA today and start with PCRs tomorrow (or maybe today). |
In general terms, the kit has a standard protocol in manipulating phages. what changes is the anion exchange column. the protocol is a bit large, but time till getting purified DNA is a few hours : like half a day. | In general terms, the kit has a standard protocol in manipulating phages. what changes is the anion exchange column. the protocol is a bit large, but time till getting purified DNA is a few hours : like half a day. | ||
Line 576: | Line 568: | ||
It seems that the best way to centrifuge the mixes is in a supercentrifuge and an ss-34 rotor. | It seems that the best way to centrifuge the mixes is in a supercentrifuge and an ss-34 rotor. | ||
- | October 7, 2009 | + | =='''October 7, 2009'''== |
Results from kit DNA isolation.- no DNA was seen in any of the fractions. There are many possible reasons, but the most likely ones is 1 .- the phage titer and 2.- the procedure bumps. everything will be clear in one more attempt and with a positive control. | Results from kit DNA isolation.- no DNA was seen in any of the fractions. There are many possible reasons, but the most likely ones is 1 .- the phage titer and 2.- the procedure bumps. everything will be clear in one more attempt and with a positive control. | ||
Line 588: | Line 580: | ||
Gel electrophoresis.- The gel with the purification fractions is considered a complete success. Although the band seen is really thin and a bit difficult to see, the size is precisely the expected one. One thing to learn about the gel is that a high voltage and more time are required. Next time, I will try running the gel for 1:30 hrs and at 80 volts. | Gel electrophoresis.- The gel with the purification fractions is considered a complete success. Although the band seen is really thin and a bit difficult to see, the size is precisely the expected one. One thing to learn about the gel is that a high voltage and more time are required. Next time, I will try running the gel for 1:30 hrs and at 80 volts. | ||
- | Given that result, I was motivated enough | + | Given that result, I was motivated enough to run a PCR for the essential and non-essential parts of P4. The essential part is a bit over 7 kb, and the non-essential part is around 3 kb. So the PCRs were performed this way: a reaction for each of the samples containing the template band, namely DNA1, which comes from centrifuge tube 1; DNA2, from centrifuge tube 2; Fraction 5 of the purification, the elution from the column, also had the band present. |
one set of reactions attempts to amplifies P4 essential, and the other one, the non essential region. therefore, I prepared stocks for six reactions (3+3 with different primers each) and a negative control with the 7kb primers. I used lots of DNTPS so my reaction won't run out of them. | one set of reactions attempts to amplifies P4 essential, and the other one, the non essential region. therefore, I prepared stocks for six reactions (3+3 with different primers each) and a negative control with the 7kb primers. I used lots of DNTPS so my reaction won't run out of them. | ||
- | October 8, 2009 | + | [[Image:Nandogel1.jpg|200px]] |
+ | <br> | ||
+ | lanes 5 and 6 have a really dim band around 11 kb. | ||
+ | |||
+ | =='''October 8, 2009'''== | ||
The Gel electrophoresis of last night's PCR has practically failed with both primer sets. Though we cannot discard the fact that the polymerase itself didn't work due to lack of positive controls, lanes of the essential region for sample DNA 1 shows two blurred spots at the size of the template at the expected size of amplification (7kb). It's not overkill to try again changing some parameters, like the polymerase or the annealing time. | The Gel electrophoresis of last night's PCR has practically failed with both primer sets. Though we cannot discard the fact that the polymerase itself didn't work due to lack of positive controls, lanes of the essential region for sample DNA 1 shows two blurred spots at the size of the template at the expected size of amplification (7kb). It's not overkill to try again changing some parameters, like the polymerase or the annealing time. | ||
Line 625: | Line 621: | ||
The result of concentrating the phage DNA from the resting elution was completely successful. The band can be seen completely at the corresponding size and the concentration is considerably high. Restrictions and PCRs will be made with this new stock. at 9 o'clock, the restriction time will have ended. | The result of concentrating the phage DNA from the resting elution was completely successful. The band can be seen completely at the corresponding size and the concentration is considerably high. Restrictions and PCRs will be made with this new stock. at 9 o'clock, the restriction time will have ended. | ||
- | =='''October | + | =='''October 10, 2009''== |
+ | [[Image:Nandogel10.jpg|200px]] | ||
- | + | Lane 8 shows the EcoRI restriction of the P4 genome. | |
- | |||
- | + | There's something really strange going on in the restriction. Even though the DNA was considerably concentrated, after restriction with EcoRI nothing can be seen, not even the template DNA. | |
- | + | ||
- | + | ||
+ | There's a possibility that the DNA, thanks to the reagents added in the restriction, runs away from the lane. | ||
- | + | =='''October 13, 2009'''== | |
- | + | So yesterday I purified DNA again, this time enhancing the technique as mentioned when I started it. | |
- | + | ||
- | + | ||
- | + | ||
- | + | The results of each DNA containing tube are here.- | |
- | + | [[Image:Nandogel13.jpg|200px]] | |
- | + | At the left we see the steps pre-protein denaturing. between the ladders, we observe all the DNA contained in tubes from 1 to 5. tube 3 was spilled before centrifugation, so some DNA was lost. Tube five contains a real lot of DNA, so let's hope it helps see the digestion. | |
- | |||
- | + | =='''October 14, 2009'''== | |
+ | Digestions were planned once again for EcoRI alone. Two more were made ith NotI and boh NotI and Xba. | ||
- | + | the expected bands for NotI alone are 4.5 kb and 7 kb | |
- | + | The expected bands for NotI and XbaI are: +-2.3 kb, close to 5 kb, a 1.2 kb band and the NotI 4.5 kb band. | |
- | |||
+ | [[Image:Nandogel14.jpg|50px]] | ||
- | + | The first three lanes are what matters. First observation.- the DNA sample added to the restriction was of low concentration, what c | |
+ | 1.NotI | ||
+ | bands observed.- | ||
- | + | +- 11.5 kb.- entire genome; incomplete restriction. | |
+ | +- 7 kb | ||
+ | +- 4500 kb | ||
- | + | conclusion.- totally consistent | |
- | + | 2.NotI, XbaI | |
+ | +-11.5 kb,.- incomplete restriction | ||
+ | seemingly 2 bands below 4 5 kb and over 4kb | ||
+ | no clue about the 2.3 b, but there could be a band around 1000-1200 b | ||
- | + | conclusion.- almost completely consistent. maybe the 2.3 kb band was somehow inefficiently cut. | |
- | + | 3.EcoRI | |
- | + | This cut better than the others since there is less initial DNA and the DNA illumination is a bit fuzzier. | |
- | + | What can be seen is a clear 8 kb band, a bit bright spot at 4.5 kb, and a 3 kb band (almost unseen). | |
+ | So this is consistent (though not evidence) with the other restriction patterns. For now, let us assume that the P4 genome does behave like it should du to the quality of the bands, which don't let us discard the alternative hypothesis. | ||
- | + | Once with a good quantity and clues about P4 presence, there are less things to control for in the PCR. | |
- | + | =='''October 15, 2009'''== | |
- | + | Today I came really early to start the protocol for chemically competent [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] and [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] cells. The idea is use the for transformation of the cox+ogr plasmid and activate with IPTG to look for phage production as plaques. These strains have to do with P4: one assesses its production and the other one has it lisogenic along with P2. | |
- | + | Other thing I did today is revisit the only aparent PCR product I obtained. It was from September 9. [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] was used for a PCR containing 2 sets of primers: P4 int and ogr. The bands expected were 300 bp and 3000 bp, but the band that appeared was of 700 bp and it's quite clear. We first had discarded this as something secondary, but it didn't contradict the possibility of having a good PCR with the correct primers used. What lacked in that experiment is more combinations of DNA and primers to consistently advance with the next part. | |
- | + | In response, I have planned and prepared another PCR reaction in which I prove all the primers against [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] and contrast with the results observed in the P4 sid1 genome. | |
+ | Conclusion: don't fear repeating a suspicious experiment!!!! | ||
- | + | October 16.- Finally the suspition is over. I ran the PCR gel for testing P4 and P2 inside [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]]. Here it is.- | |
- | + | [[Image:Nandogel16.jpg|200px]] | |
+ | Lanes. | ||
+ | 1negative control (no DNA) | ||
+ | 2 cox | ||
+ | 3 ogr | ||
+ | 4 [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] +int | ||
+ | 5 ladder | ||
+ | 6 [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] + P4 | ||
+ | 7 [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] INTp4 | ||
+ | 8 P4 DNA P4 | ||
+ | 9 P4 DNA | ||
+ | 10. p4 DNA INT p4 | ||
- | + | So the mysterious band is still present... well. another experiment variation is to use different combinations of primers. I have set the PCR to come out tomorrow. let's see what happens. | |
- | |||
- | + | =='''October 17, 2009'''== | |
- | + | I ran the gel testing different combinations of primers. there was no product either, so after all, we can conclude that the primers don't work. It has always been strange that both pairs of primers wouldn't work, but it seems to be the case this time. Final possibilities for lack of function.- | |
- | + | 1. there is no phage DNA. The restriction assays don't show this, neither does the +- 11 kb band in the gel. | |
- | + | 2. there are no sites for both primer sets.- valid option | |
+ | 3. the genome is an isomorphism which doesn't allow amplification because of primer orientation.- at least some incomplete products should be seen. | ||
- | |||
- | + | =='''October 19, 2009.'''== | |
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
+ | Yesterday I transformed [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] and [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] cells with plasmid 18 + cox and ogr under the control of a lac operator. [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] where the only resistants obtained, and negative controls are valid. So it's time to plan the experiment to validate the presence of cox and ogr inside the bacteria. It cannot be done from direct PCR, since [[Team:LCG-UNAM-Mexico/Resources/Strains|C2423]] already had both genes. It cannot be done only from plasmid extraction, unless the precise band is checked. the best method would be extracting plasmid and performing PCR to it. At the same time, plating on IPTG plus controls will be done, eventhough it is not sure that it will work. The expected results are P2 plaque formation. Too sad that [[Team:LCG-UNAM-Mexico/Resources/Strains|C331]] didn't transform, because we cannot observe direct interaction with P4. So growth experiment will be as follows.- | ||
+ | for a plasmid containing colony, there will be these plates.- | ||
+ | simple LB | ||
+ | LB with IPTG | ||
+ | simple LB added .1 M IPTG on half of the plate. | ||
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Latest revision as of 02:56, 21 October 2009