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Selection of ssDNA Aptamers for Use in Detection of Cancer Biomarker-Carcinoembryonic Antigen

According to Qiagen kit the primer concentration for PCR amplification should be 0.5uM. So I did PCR amplification for primer concentration that we have been using and primer concentration according to Qiagen protocol. PCR amplification worked only with 20uM primer concentration.

Conclusion: keep using primers that you have been using

Problem: still having multiple bands

Preparation for SELEX 9; PCR optimization: cycles 10, 12, 15 and 20

To resolve problem with multiple banding I decided to use two different cycles 15 and 20. Then I further gel purified band from 15 cycle run.

Conclusion: In 15 cycle PCR amplification program there is less by product comparing to 20 cycle PCR amplification program

Problem: Still having multiple bands

After gel purification of SELEX 8 product, I have set up another PCR amplification, but this time with 10,12 and 15 cycles. According to the image cycles 10 and 12 gave less by products whereas cycle 15 didn’t. I have used two set of DNA template for cycle 15: first from SELEX product 8 and second from SELEX product 8 that was gel extracted. This time gel extraction didn’t gave us anything exciting.

Conlclusion: Gel extraction method didn’t work this time. Use cycle 12 for further PCR amplifications.

2. SELEX 7-12 RESULTS

CONCLUSION:

12 cycles of SELEX procedure were completed successfully. The next step is analyze their affinity to CEA using DOT-Blot Assay. Also start to clone SELEX 11 and 12 products into E.coli.