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PCR--RT-PCR-and-Real-Time-PCR
211.
PCR with more than one primer -
(reply: 1)
212.
RAPD - PCR problem -
(reply: 5)
213.
Relative fold expression and Normalization fold expression -
(reply: 2)
214.
Strange Bands -
(reply: 2)
215.
Recommended tamplate DNA concentration for qPCR -
(reply: 2)
216.
RT / cDNA synthesis -
(reply: 7)
217.
How to best store PCR product? -
(reply: 2)
218.
smearing below band of interest -
(reply: 5)
219.
RT-PCR primer design -
(reply: 1)
220.
After PCR, One Band on 1.2% Agarose but 2 bands on 8M Urea, 8% PAGE -
(reply: 1)
221.
Odd gel run following PCR -
(reply: 28)
222.
Qiagen PCR Array Reagents? -
(reply: 1)
223.
Enough checks for gDNA contamination in qPCR? -
(reply: 3)
224.
plate stuck in ABI7300 -
(reply: 7)
225.
No or very weak band using 16s primers -
(reply: 1)
226.
No PCR amplification with b-actin primers -
(reply: 1)
227.
Is PCR efficiency higher if mutation is in the middle of primer? -
(reply: 7)
228.
optical qPCR plates -
(reply: 1)
229.
Fold change significance -
(reply: 2)
230.
No PCR amplified with long primers -
(reply: 10)
231.
How many real time-PCR reactions for statistics and how? -
(reply: 4)
232.
PCR optimization: PCR vs qPCR -
(reply: 4)
233.
PCR smear for genomic samples -
(reply: 4)
234.
Smaller band appear under Main product with every primers sets from PCR -
(reply: 3)
235.
Saliva and GCF DNA purification -
(reply: 1)
236.
rtPCR working but the elongated product wont gel! -
(reply: 1)
237.
another primer dilution question -
(reply: 2)
238.
TaqMan qPCR low-template issues -
(reply: 1)
239.
qPCR standard curve slope (m) -
(reply: 2)
240.
16s double bands obtained-why?? -
(reply: 2)
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