Primer designing

I was studying this subject and couldn't understand why the reverse primer was the complement reverse of the leading strand. Now I got it, thanks to your awesome explanation. Thanks!!!

thank you so much. a 4 hour lecture in class did a horrible job of explaining what you explained so easily in 20 minutes. thank you

You saved me as I am studying for the final examination... thank you so much

Thank you so much for this thorough explanation! It helps a lot.

Thank you very much for this informative tutorial! Congratulations on the good work!

The way you explain this things Shomu. So helpful

Viewing from Kenya, with an example coming; you are really a saviour Sir.

Thank you very much. It's very clear. This RTD helps me a lot.

amazing..thanks a lot for making me understand this process for the first time.

Thank you very much. Very informative and helpful. Congratulation!

This was very helpful, thank you for sharing.

Your explanation is better than my lecturer !!! Thank you so much, u save my final paper tmr !!!

Dear Shomu, Thank you for the video above, it was quite helpful. I am having trouble designing new primers for HDV genotypes' G1-G8 and G1,2,4. How d I go about doing this? I have tried using NCBI.

this is very good suman. it is the easiest way to explain primer design
thank you

Thank you very much. It helps me understand this within 30 min.

Thanks Shomu! You're basically saving me on accomplishing my master degree hahahaha!

Thank you sir i always see you lectures when cannot under stand the topics .thuk you so much.
may God bless you with happiness and success in life.

Hello Shomu, thank you for your videos, I got a question, I designed a pair of primers to amplify one region of a 3200 bp gene. But after sequencing, some samples yield one section of the gene and others yield other section of the gene, do you have an explanation for this? thank you.

Its really cool. thank you very much for helping others.

thanks brother for such explaining , you are great

Great Shomu. You are the best

u made my life easy!!!!!! thanks a bunch!!!

nicely explained. Best teacher for Biology and biotechnology

Wow ......powerful explanations.....this is really cool

Very well discussed in the shortest possible time Shomu. aaro video koro. sabash.

Decent summarization of the topic. How about a video on the proper step by step design of primer. A simple tutorial

I was wondering about the melting temperatures for the primers? For example, if one primer has a melting temperature(Tm) of 55 and another a Tm of 65. Say I lower the temperature to 60. Wouldn't the 65 Tm primer anneal but the temperature of 60 is still too high for annealing?
So if I want both primers to anneal, don't I have to lower the reaction temperature to the lower of the two melting temperatures to get BOTH primers to anneal?

Best one you are for me sir ..... literally ......Thank you so much sir 😊😊

tq so much.. it helps me understand this within one night...

Amazing brain!! So helpful...appreciate ur knowledge level

Very thoroughly explained. Thank you for sharing💝

Thanks a lot but I am not clear with the "distance between base pairs" I just got confused as to how do we manage that?

Thank you for your simplest explanations ❤

Thanks for sharing !

Thanks a lot ... that was well explained and brief :)

Thank you sir.Very good explanation.

Excellent video.

thank you soo much it was really helpful

U saved my Final paper man... Thanx

Can u please do video on how to select primers in NCBI and how to do blast ? What are the mistakes to avoid?

Best explained....thanks sir

Its realy vvv well done.. but I have one question..please.. How to add the restriction sites?? if we are going to design primers for cloning- Gene construct..??????????????????????

Thanks so much sir. I love you. U simplify my work ❤️❤️❤️❤️❤️❤️❤️

Thank you sir I got it a lot of knowledge from your video actually I work in molecular laboratory

Hello sir I've got a query, as you've said during the lecture that primer will be used to amplify the gene of our interest, so it means that we will design the primer according to our gene sequence, so my Q. is how to the identity that gene and its sequence?

Thank you !

Thank u very much.

I want to know if the extension temp is 72 and annealing temperature is 54,so at this high temp of 72, the primer and our DNA strand should denatured but this never happens.why??

amazing video...
my question is how to get to know these information e.g melting point of a specific primer?

Hii, Which software you are using?

thank u very much, it's very understandable and informative

why are you so smart? :D thanks for the explanation

very lucid way of pesentation

Sorry, but you're completely wrong about one of the primers not binding if the temperatures are not matched. You give the example of one primer with a Tm of 55 and another of 65. You state that if you use 55 as the annealing temperature, the Tm 65 primer won't bind at all. This is incorrect. It will bind. However, as the temperature decreases to below 65, there is an increased opportunity for non-specific binding elsewhere in the template which could lead to inefficient PCR and/or artefactual amplicons.

Very helpful, thank you so much

can you please make video for control of PCR contamination

Thanku so much, it is so helpfull

Fir the primer diner they only form the dimer if the three from the end were consecutive meaning from 3’ end sequence they would have to be 3 in a row no gaps to form a primer dimer

Very informative

Good morning sir
Can you please tell me if short primer gives unwanted binding then what happened with out of range very long primers??

Jazakallah sir..., 👍💖
Form Pakistan

I didn't get it. Did you mean annealing temperature instead of melting temperature ?

good one

thanks alot

Love u sir 💗💗

excellent

Sir can you please explain the difference between runs and repeats and secondary structure. Thankyou ✨

Great video 🤗☺👍

how to i download this video ?

Sir, pls clear what will happen if we have 90%GC content??
🙏

Great video, but I didn't really understand the bit about melting temperature. If you're denaturing the DNA at over 90 degrees C, but the melting temperature of the primers is 50-something to 60-something degree C, what stops the primers from being damaged? Does that make sense? Is it because the melting temperature breaks the hydrogen bonds? In which case, why does heating the reaction up again to over 90 degrees not break the bonds and damage the primers? That's the one thing that has me a bit confused. If anyone in the comments section knows, I'd love to have the answer. :)

Thanks

What is gen ?

excelent

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thank u

BestOne

👍

I have a question it may be a stupid one butt sir everything else is fine, but after designing pimer, from where do you put the primer in the tube, remove it from the computer or what?

I wonder what is your education level?

😍

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Thanks

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