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PCR--RT-PCR-and-Real-Time-PCR
211.
How to set up real-time PCR for yes/no bands (rearrangement) -
(reply: 4)
212.
RNA concentration is too low to detect gene of interest by qRT-PCR -
(reply: 4)
213.
RT-PCR help -
(reply: 2)
214.
Strange signals in the NTC -
(reply: 1)
215.
False positive - help -
(reply: 3)
216.
Autoclaving PCR waste in the room where PCRs are set up and run - Is it a proble -
(reply: 2)
217.
PCR Temperature change control malfunctioning -
(reply: 1)
218.
Assay question -
(reply: 1)
219.
WHY NO ONE REPLIES, is this a stupid question ? -
(reply: 5)
220.
HRM instrumentaion -
(reply: 4)
221.
Can you repeat a thermocycle? -
(reply: 3)
222.
Any online tool to check the propability of primer dimer formetion _ -
(reply: 4)
223.
Amplification curve in the negative control samples -
(reply: 7)
224.
PCR troubleshooting: wrong amplicon size when spiked into sample -
(reply: 4)
225.
Primer as limiting reagent in PCR reaction -
(reply: 2)
226.
Taqman probe in a LightCycler 480? -
(reply: 1)
227.
Real time PCR for degraded RNA -
(reply: 1)
228.
Ct value of housekeeping gene -
(reply: 4)
229.
Efficiency correct fold change -- use all or none? -
(reply: 1)
230.
Microfluidic PCR Issues, Master Mix and Consumable Variations? -
(reply: 5)
231.
Doubled polymerase in the rxn, does this increase pcr efficiency? -
(reply: 1)
232.
If I am running Real-Time PCR with one gene of interest and one reference gene(G -
(reply: 4)
233.
Do I need to run HKG together with the GOI everytime I run Real-Time PCR? -
(reply: 1)
234.
Is this primer-dimer peak in my melting curve? -
(reply: 6)
235.
Taq / Phusion mix -
(reply: 3)
236.
I'm working on an automated DD2CT value generator for Life tech qPCR machine -
(reply: 2)
237.
Dilution series between HKG and GOI -
(reply: 7)
238.
Reference gene(s) selection and validaton for qPCR -
(reply: 5)
239.
Is that normal the negative control showing signals? -
(reply: 13)
240.
qPCR cannot detect reaction. -
(reply: 1)
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