Primer designing for real time PCR using NCBI Primer Blast

  Рет қаралды 167,227

Bio-Resource

Bio-Resource

Күн бұрын

This video explains how to design primers for real time pcr using primer blast.
NCBI's primer blast tool helps in designing primers and also allows to check the specificity of the designed primers.
Various options are available to improve the primer stringency.

Пікірлер: 39
@annavl4937
@annavl4937 4 жыл бұрын
Hi, thanks for the video! Another way I know to avoid potenitial genomic DNA amplification is by selecting "Primer must spand the exon-exon junction", so no intron-including DNA would be amplified.
@sanjuktaghosh8802
@sanjuktaghosh8802 7 ай бұрын
Hi, a very useful video. Could you link the video in which you have discussed how to increase stringency so that the primers become more specific. Kindly reply :)
@papajiang8487
@papajiang8487 Жыл бұрын
I am wondering how does this tool guarantee the primers are specific to human? Can I say once you input the organism option as human, then the tool will help you to design specific primers to human? And if the primers only have one SNP to a different species, does it still call specificity just due to the one SNP?
@murchanabarua7168
@murchanabarua7168 Жыл бұрын
I have a question? Using this website how would I make a forward and reverse primer that is 18-35 nucleitodes long? because whenever I put that into "PCR product size" from min 18 to max 35 it doesn't work.
@kulkuljator
@kulkuljator 28 күн бұрын
Thank you so much! Once I returned home from the lecture, I realized that I do not remember shit.
@Scienceiirwn
@Scienceiirwn 4 жыл бұрын
Amazing Video!!! Is there anyway you can do a video on designing a primer to target different variants ? for example i noticed in your example there are many GAPDH variants (V1 -V4), what if you want to target the different variants to see the expression of each one? I would really appreciate if you can give an example using CD44 which has 10 variants.
@beinghuman4457
@beinghuman4457 9 ай бұрын
sir i have a confusion ? when we have to select nucleotide and when we have to select gene in the database ?
@anuranjanapv4484
@anuranjanapv4484 3 жыл бұрын
Hello sir, thank you for the video! How to select the variant of our gene of interest? On what basis we have to choose?!
@anishamn2172
@anishamn2172 Жыл бұрын
How you assign a particular value to Tm. What is the criteria for that value?
@AZMERANDA24
@AZMERANDA24 2 жыл бұрын
Thank you for the video, my question is, what I should do if the primers were not found? Is there another way to design primers?
@BioResource
@BioResource 2 жыл бұрын
Hi +Dina Human, You can relax the parameters / stringency or input the region of interest and try using primer3. Hope this helps.
@h1bB0ilzZ
@h1bB0ilzZ 2 жыл бұрын
Thanks for the video, it was very helpful. Is the process the same for qPCR primers?
@egamberdimaxmudov1676
@egamberdimaxmudov1676 11 ай бұрын
How can I record laptop monitor that I design primer ?
@chi-kandy
@chi-kandy 2 жыл бұрын
I want to run a primer blast for a microorganisms, how do I run the DNA sequence?
@raselkhan1384
@raselkhan1384 2 жыл бұрын
Have you figured it out? I'm struggling to validate some of the primers for resistance genes that I collected from literature.
@krishnaprasad5508
@krishnaprasad5508 9 ай бұрын
Thank you very much. It was beautifully explained.
@palakmehta8820
@palakmehta8820 5 ай бұрын
Hello sir.. I am trying to make primer for plant sample. Itried to do as shown in the video but it is showing error like. The primer specificity can not be determined as sequences for the selected organism are not present in selected database: refseq_mrna please help me with this.
@somayehmohammadi7794
@somayehmohammadi7794 3 жыл бұрын
Hello .How to be extract PSSM profiles and to be generates matrix? I have consider linear substitution probability matrix.
@mohammadrezasamiee5669
@mohammadrezasamiee5669 3 ай бұрын
Hi thanks for the video, but I didn't see probe for real time pcr
@adeshkolekar3425
@adeshkolekar3425 4 ай бұрын
HELLO SIR ITS TAKING TOO MUCH TIME TO GET THE RESULT CAN YOU PLEASE HELP TO SOLVE THIS ISSUE
@bijayininayak2100
@bijayininayak2100 Жыл бұрын
How to do primer sequencing in plant gene
@ayeshamalik456
@ayeshamalik456 2 жыл бұрын
Hi, thanks for this wonderful Video. I learnt a lot from your videos. Can you please make a video on how to analyze sanger sequencing through Geneious Software and MEGA? Will be much Appreciated. Thanks
@KimiaGhadiri-qu1ev
@KimiaGhadiri-qu1ev Жыл бұрын
Hello , thanks for your explanations . I wondered if i can ask some questions . Iam a total newbie in PCR . I used Perlprimer app for making primer for CFTR gene but the result in NCBI site for my primer was different with the app eventhough i considered the same situation for both can u please help ? 🩵
@biologywithboss8296
@biologywithboss8296 5 ай бұрын
Sir some problem please help me RT PCR primer design
@yunasali5642
@yunasali5642 2 жыл бұрын
sir, i want to know about entrez query
@guihuajia7696
@guihuajia7696 Жыл бұрын
very good video for people!
@BioResource
@BioResource Жыл бұрын
Thank you. Consider subscribing 😊
@prabhubiograd
@prabhubiograd 3 жыл бұрын
The video must have included probe design too in case of real-time PCR
@deenadeena5305
@deenadeena5305 2 ай бұрын
Yes, kindly include that video too!
@r.seenaiah
@r.seenaiah 2 жыл бұрын
Good information
@Achilles189
@Achilles189 4 жыл бұрын
Are you malayali
@gehadmahmoud6058
@gehadmahmoud6058 4 жыл бұрын
Very nice explanation. Thank you :)
@IkanPediaMalang
@IkanPediaMalang 4 жыл бұрын
nice explanation...
@alpmogulkoc9148
@alpmogulkoc9148 3 жыл бұрын
thanks really helpful
@ogunoluwamayowa4749
@ogunoluwamayowa4749 4 жыл бұрын
Lovely, thanks
@mohamedsal_traiki6954
@mohamedsal_traiki6954 4 жыл бұрын
Dankeschön
@yossiepdrn8933
@yossiepdrn8933 4 жыл бұрын
Thanks!(:
@drrakeebahmad8736
@drrakeebahmad8736 Жыл бұрын
Great
@BioResource
@BioResource Жыл бұрын
Thank you. Consider subscribing.
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