I'm having to give an R coding walk-through to some Stanford first years on Wednesday, and it had been so long since I'd done any qPCR I had forgotten the details. This video was perfect. Thanks for making such a well organized, clear and informative video.

Great video! I went through 5 other videos that were either too simple, way too drawn out to keep watching, or ended up being sales pitches for certain reagents or instruments.

eventually however enough amplified product accumulates to generate a 1:22detectable signal the cycle number of which this occurs is the threshold cycle 1:27or CT in this plot the threshold fluorescence is indicated by the green 1:32line in real-time quantitative pcr the data that are generated are the 1:42threshold cycle or CT values the threshold cycle is determined mainly by 1:48the amount of template present at the start of the amplification reaction if a 1:52large amount of template is present at the start of the reaction relatively few

Your content is so touching

What do you do when the control Ct is undetermined, like in a case of transgenic line versus WT where a foreign gene is undetected in the WT.

I didn't take any control gene,how to calculate delta delta value now? suggestions plz

Shouldn't we take the ratio as calibrator/test instead of test/calibrator in order to conclude that expression of the gene is 8-fold higher in tumor cells, since the ratio of 8 indicates that "test"/tumor cells have higher CT, thus lower expression? I'm just checking because I'm new to the subject, I'd appreciate it if someone could answer :)

Great explanation. Thank you very much!

if we want to know significant value from expression gene by statistic. What should i have to input in spss? Value from 2-∆∆Ct from sampel treatment and control? Or value from ∆CT sample and control

So in absolute quantification, you determine how many copies of the sequence are in your sample, but how would you translate that information into how many copies are in the genome?

What is the app which help to take a video?

how did you do it can you share with me , thank you

HBV DNA detected within the liner range of the assay means

Hello. Can anybody help me to calculate how much fold increase/decrease in gene of my interest occurred as a result of my compound treatment. I have been trying to sort it out but couldn't . Ct values for GADPH and WNT of control group are 14.3292 and 22.274 respectively, while Ct values for GAPDH and WNT in treated group are 14.1418 and 23.9879 respectively. Please help me to reach to the conclusion. Regards!

At the present, My Piko Real PCR system (Thermo Scientific) had E36 error (Strain gauge has problem). Could you help us to solve the error? Hope to get your feedback.

can i use this relative quantification method in telomere length by using ratio

when i go for absolute quantification of DNA, after the experiments green coloured flags are apperas on it, along with standard samples and with unknown samples, may i know why this happens sooo ? i am using ABI Stepone plus ver2.2. kindly help or suggestions r welcome

very helpful thanks

I ve got some results with + not in mince what does that mean

may i know what is the unit of quantity while quantification of pathogen load ? another how to convert teh absolute data into to copy no. of the pahogen.? kinldy help urgently

How to calculate log value.

Thank you

very clear

How can i know the efficiency is 100%.

Why is it truncated this video? what about the normalization against the reference gene? Since is actually the video of another video (BioRad's ?) you could have referentiated it, right? Disappointing...

Thompson Robert Wilson Jose White Deborah

R.T PCR with milk samples

thank you very much

Hello! Can I help you translate this video to Spanish?

Nice! Thank you :)

interpolate, not extrapolate!

Please help Bio-Rad

Dat voice

not helpful at all

You are exerciseng torture on living men and women this breaking every law and legally any were in world or iso or any digit sumbal place of existence