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Silvia_84

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  1. Hi all, I got nucleotide sequences of a PCR product corresponding to a specific variant of an enzyme I am studying. I made a search of homologies by BLAST to see if the gene I have shows 100% homologies with already known variants or if it is a new variant. I found some changes in the sequence and I would like to know if this change is just a silent mutation or it leads to a different amino acid sequence. How can I check this? Do you know good softwares for the translation of the DNA sequence in amino-acids? Thanks
  2. Hi all, I am new in Microbiology lab and I was reading about the conjugation assay that is done to see if the resistance is transferred among bacteria. I was wonder..can this test work if the plasmids are not transmissible? How reliable is this test in testing if the plasmids are transferred?Do you have an idea? Any suggestion is appreciated. Thanks
  3. Hi all, could you explain to me why the carbapenems (and other antibiotics) are considered last-resort drug? I am aware that they are used when all the other drugs fail to treat infections but I don't understand why they are the strongest..Do they have more catalytic activity?Do they act with particular molecular mechanisms?Can you explain me please? Any suggestion would be really appreciated. Thanks
  4. Hi all, can anyone suggest me a method-protocol to understand if a gene is on the genomic or plasmidic DNA?I have done PCR on purified DNA (that is both genomic and plasmdic)and I found the gene I was looking for. Now I would like to understand if this gene is located on the plasmid or on the genome. How can I do that? Thank you
  5. Hi all, I tried to do multiplex PCR to amplify more genes at once with the biomix red polymerase. Unfortunately it did not work (no bands at all, not even primer dimers)and I have no idea of what goes wrong. The primers should be ok because I am using those already used by another group who has already done the same multiplex PCR.I don't ' know if I make some mistake in the procedure: For a 25 ul of reaction mixture I added: 12.5 ul of BIOMIX RED 1 ul of each primer (they are in total 8 because the genes I am amplifying 4 genes together) 3.5 ul of water The single PCR, done with the primers separately is fine.. so there must be something wrong in the multiplex set-up Thank you in advance.
  6. Hi all, I have some stocks of bacteria frozen with beads. I was wondering what method is used to streak the beads on the agar plate.Do I need to shake a bit the plate to let the beads rub on the agar?Or are you aware of other more accurate techniques to do it? Thank you in advance.
  7. Hi guys, I have two questions about the preparation of bacterial freezer stock with beads.It is new for me. How can I make it?Can you indicate me the procedure/ steps to carry it out? When I have to streak the bacteria from the frozen beads , how is it better to do it? roll the beads on an agar plate or just use a loop to touch the beads and pass it on the plate? Thank you very much.
  8. Hi all, I am doing PCR and I am using the biomix red as a polymerase. The mix already contains all the components for the reaction but I need to increase the concentration of magnesium in my reaction. I can't understand very well the protocol. It says that the MgCl2 concentration in the buffer provided is 6mM (3mM final concentration) and should be adjusted just if necessary. Then it reports a table showing the volume of additional MgCl2 to add to a 50 ul reaction to achieve different final concentrations. The table says to add 0 ul of 50 mM MgCl2 to 50 ul final reaction volume to reach a concentration of 2mM, 0.5 to reach a concentration of 2.5 and 1 for a 3mM concentration. What I don't understand is that reading this protocol it seems to me that the reaction mix already contains 3mM of Magnesium. So why should I add 1 ul to reach a final concentration of 3mM?And if I wanted a 5mM concentration, should I add 3ul? I was not able to attach the link, anyway if you google biomix red protocol , you find it right now. I hope to have been clear. Thank you
  9. Hi guys, can I ask what I should do if I want to order some bacterial control strains for PCR? What is the procedure? Do I need the genomic sequence of these strains?Are there websites for this? Thank you very much
  10. Hi all, Do you have experience in multiplex PCR? Do I need a specific polymerase for this kind of reaction? Thank you,
  11. Hi all, I extracted DNA and now I have a stock solution in TE buffer and two aliquots in water. How is it better to store all these solutions since I need to use it for long periods of time? Freezer or fridge? Thank you
  12. Hi all, I have to do PFGE on some strains of Klebsiella. It is the first time I do it and I am reading a protocol for the prepararation of agarose embedded bacterial DNA. The procedure says at a certain point to remove 5 X 108 cells (I suppose they refer to a bacterial suspension) for each ml of agarose plugs to be made. Can you explain me how you determine the volume of bacterial suspension corresponding to this amount of cells (5 X 108) and how is it calculated? I need to know it even for other protocols that say to take a specific number of cells and I did not understand how to convert this amount in volume. I thank you very much.
  13. Hi all, I have to run a PCR reaction and I am following a protocol suggested by the company of the TAQ polymerase I have. The protocol says to use 10 ul of 5x MyTaq Reaction Buffer and 0.25 - 1 ul of 2XTAQ polymerase. in the reaction Does it mean that I have to diluite both before using them since they are concentrated respectively 5X and 2X? Or shall I take the amounts suggested by the protocol from the concentrated solutions as provided by the company? It is not specified on the protocol.. Furthermore, I did not understand very well how I can calculate the volume if TAQ polymerase I need if the concentration is reported in Units.. e.g. If the protocol says to add 1.25 units of TAQ, at what volume does it correspond?Can you explain me a little bit the calculations I should do? Thank you very much in advance
  14. Hi all, I was wondering if you can illuminate me or give me some opinions on what can go wrong during my PCR reactions. I extracted bacterial DNA and I diluited my DNA samples 1:10 and 1:100. I tried to run different PCRs to identify a gene. I run a PCR by using the extracted DNA as it is, another one with the DNA diluited 1: 10 and another one with DNA diluited 1:100. I was able to see the product if the DNA was dilutied 1:10 and 1: 100, but not if I used the extracted DNA as it is. I thought that maybe something with DNA extracted during the PCR reaction can go wrong because the DNA is too concentrated, since in the other two cases (when DNA is diluited) it works ...does it make sense for you?Or do you have other suggestions? I tried to run again these same PCRs, same conditions but this time I am able to see the product with the DNA extracted and when it is diluited 1:100 but not if it is diluited 1:10...Do you suggest something?What would it mean? Thank you in advance
  15. Hi all, Do you usually centrifuge your samples containing the mix for the PCR before running it? Thank you in advance
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