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<IMG_20161218_091257.jpg>
What makes you think it did not work ? I did not have any dots at the beginning, now there are, so something is growing.
It definitely looks like you have growth in both sides of the plate. The bottom doesn't have dots because the growth is too thick to see gaps between the colonies.
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It definitely looks like you have growth in both sides of the plate. The bottom doesn't have dots because the growth is too thick to see gaps between the colonies.
On Thu, Dec 22, 2016, 5:38 PM ukitel <marco.r...@gmail.com> wrote:
I'm afraid there is no streptomycin on the plates.
Can you describe in detail how you made the plates?--
On Thursday, 22 December 2016 20:20:47 UTC+1, Hugues wrote:Hi guys,i think i have successfully CRISPRed an E. Coli bacteria,I have used the kit sold here:I followed the protocol here:The gene that was targeted is Escherichia coli 30S ribosomal subunit protein S12 (rpsL) gene. One base pair was changed to render the bacteria resistant to streptomycin.The picture attached shows my result. That plate contains a gel with streptomycin. The top part shows growth on the CRISPRed strain, the bottom part shows not growth on the normal strain.What you guys think ?I'm thinking of having the DNA of that gene sequenced, just to check if the edit really happened only where expected.
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This hypothesis should not be too difficult to test.Perhaps viewing the non-dot areas under a microscope (perhaps with a stain for that species) would quickly find individuals, or taking a small sample of that area and streaking another plate to see if colonies form.Cheaper than sequencing, and faster.
On Thu, Dec 22, 2016 at 3:47 PM, Bryan Jones <bryan...@gmail.com> wrote:
It definitely looks like you have growth in both sides of the plate. The bottom doesn't have dots because the growth is too thick to see gaps between the colonies.
On Thu, Dec 22, 2016, 5:38 PM ukitel <marco.r...@gmail.com> wrote:
I'm afraid there is no streptomycin on the plates.
Can you describe in detail how you made the plates?--
On Thursday, 22 December 2016 20:20:47 UTC+1, Hugues wrote:Hi guys,i think i have successfully CRISPRed an E. Coli bacteria,I have used the kit sold here:I followed the protocol here:The gene that was targeted is Escherichia coli 30S ribosomal subunit protein S12 (rpsL) gene. One base pair was changed to render the bacteria resistant to streptomycin.The picture attached shows my result. That plate contains a gel with streptomycin. The top part shows growth on the CRISPRed strain, the bottom part shows not growth on the normal strain.What you guys think ?I'm thinking of having the DNA of that gene sequenced, just to check if the edit really happened only where expected.
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They will survive in the fridge for weeks.
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If you are not sure of streptavidin, you can add sterile strepatvidin solution on the top of the plates(0.5 ml - spread by tilting the plate), let dry.Use two separate plates, one for WT, one for mutant. On each plate streak a loopful (about 10=20ul of bacteria) using the T-method (draw a T on the back of your dish, first streak the bacteria at the top of a T (red in diagram), then sterilize the loop, and pull down a streak from the top of the T down the leg of the T (yellow in diagram), sterilize loop again, and then starting from the bottom zigzag up (green in diagram) leaving about 1 to 2 cm from the cross line of the T (a sterile zone)). Incubate, you should get single colonies.
On Sun, Jan 15, 2017 at 8:55 AM, Hugues <lalibe...@gmail.com> wrote:
so as mentioned in my last post i streaked the "mutant" and the wt onto another plate with strep,this time i took a very small qty of each colony and spread it as much as i could,As you can see in below pictures (0, +6h, +9h and +30h after streaking), initially i could barely see any trace, then both colonies grew, maybe a little less on the wt side, but i don't know if it is significative.So i would think i don't really have strep on this plate.I guess i would have to sequence both colonies to be really sure if i managed to edit the "mutant" or not.
On Thursday, 22 December 2016 20:20:47 UTC+1, Hugues wrote:Hi guys,i think i have successfully CRISPRed an E. Coli bacteria,I have used the kit sold here:I followed the protocol here:The gene that was targeted is Escherichia coli 30S ribosomal subunit protein S12 (rpsL) gene. One base pair was changed to render the bacteria resistant to streptomycin.The picture attached shows my result. That plate contains a gel with streptomycin. The top part shows growth on the CRISPRed strain, the bottom part shows not growth on the normal strain.What you guys think ?I'm thinking of having the DNA of that gene sequenced, just to check if the edit really happened only where expected.
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