Western Blot - Theory and method

Рет қаралды 218,066

Күн бұрын

Пікірлер: 54

@Vekey2 5 жыл бұрын

This video was everything I wanted! I have a vague idea of everything in here and just needed a refresher on the actual practical use of everything. Thank you!

@SerenSanguis 3 жыл бұрын

Very nice! The closest thing we have to lab practice in the pandemic!

@vishk123 2 жыл бұрын

Thank you for inviting me to your game! I played and learnt a lot!

@hirosewill893 7 жыл бұрын

Nice protocol and instruction. Thank you for the video

@RoyRahebKhelo 6 жыл бұрын

Splendid presentation, thank you.

@lincolnoliveira3041 3 жыл бұрын

Rider

@prembobby112 2 жыл бұрын

Everything clearly explained to more useful to practice this Western Blotting Thanking you Sir/Mam

@DocScoop7 Жыл бұрын

it was such an awesome video

@Lina-7578 6 жыл бұрын

Thank you! Great video, it helps me a lot!

@tle6974 7 жыл бұрын

Good video but please 14:51 dont hold the pipette upside down with a used tip on it... ;)

@travstravinho2766 7 жыл бұрын

Yas omg

@JaLLaM86 6 жыл бұрын

... Or use a computer mouse with gloves on.

@tylerlord1340 6 жыл бұрын

can you explain why?

@bradywells1293 6 жыл бұрын

The liquid can make its way into the pipette and cause contamination to the next sample(s) you use it for or it can just damage the sensitivity of the pipette by getting stuff gunked up inside.

@KalahSimpson 6 жыл бұрын

Better yet, use filter tips

@amymay16 2 жыл бұрын

Thanks, great video! How does the metal stirrer help the process? I usually leave the tank without it being stirred the whole time, would love to know how stirring it helps as I may try that! Thanks so much in advance.

@dishabanerjee9630 9 ай бұрын

Thank you so much!!

@jfromtheusa Жыл бұрын

hugely helpful

@ماجدفرج-خ4ط 6 ай бұрын

Nice video, how long for blot ting at 115 volt?

5 жыл бұрын

Very useful video. Thank you.

@BalajiHariPhD 2 ай бұрын

I'm interested to do this western blot techniques

@valentinascatizzi6406 4 жыл бұрын

thank you, brilliant and accurate explanation

@Biomeducated 5 жыл бұрын

Great tutorial! But, 13:58 you didn't depict the amplification tree (usually the secondary is polyclonal), so there's multiple secondaries binding to the primary to 'blow up' your signal from the HRP reaction. Besides that: *great channel* here, man! Why did you stop though :( Just as I'm discovering all these helpful channels... I even made a Top 10 channel overview on my own channel, and I'm planning on making a second one with 'smaller channels' like this one. All good stuff for Biomedical/Life Science students!

@lukehebert6207 3 жыл бұрын

I'm re-acquainting myself with this stuff after years of not being in a wet lab. Thanks for this detail and the overview vid on your channel. Polyclonal secondary antibodies sounds clever and makes a lot of sense.

@Biomeducated 3 жыл бұрын

@@lukehebert6207 Cheers, man!

@digitalmediazone9717 Жыл бұрын

Thank you

@SixTough 7 жыл бұрын

excellent

@Kysersozé1 3 жыл бұрын

Thank you.

@AwaisAli-xl1pu 10 күн бұрын

Hello Sir, I have facing repeated problem with my bands in WB, can you help me? Same problem persist despite of all repeated correction. Trouble shoot i am unable to identify

@汪华志 6 жыл бұрын

i have a question : how tween inhibits detection ? what is the reaction mechanism

@imranchandler1083 3 жыл бұрын

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@axtonjax3700 3 жыл бұрын

@Imran Chandler Instablaster ;)

@imranchandler1083 3 жыл бұрын

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@imranchandler1083 3 жыл бұрын

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@axtonjax3700 3 жыл бұрын

@Imran Chandler You are welcome xD

@AmandeepSingh-vc2wj 3 күн бұрын

POV: You searched this video because you placed the membrane on the wrong side and lost your sample, so you're repeating the experiment again...

@rishavdas9939 7 жыл бұрын

Good

@ChristyLuvz 6 жыл бұрын

Can the primary and secondary antibodies be diluted in the 5% non-fat milk and then each incubated with the membrane? Rather than doing the blocking step as its on whole step?

@Biomeducated 5 жыл бұрын

You mean put everything in at once at the same time to reduce protocol time? Not with the blocking step for sure, but perhaps you can premix primary and secondary at equimolar concentrations, then you are sure that no excess secondary will deplete your primary if you wash afterwards. Then again, you would loose your 'amplification tree' which could results in not seeing a good signal. Usually the secondary antibody is a polyclonal so multiple HRP-conjugated antibodies bind to the Fc-part of your primary, needed to amplify your signal. I would just stay with the sequential protocol. Or maybe I misread your question (just realized I think): yes, your antibodies should be diluted in the same solution as the blocking, but usually it's more diluted than for the blocking. So if you block with 5%, you stain in 1% or 0.5%. Note that some protocols recommend using BSA as blocking and for dilution...

@МаринаЗеленюк-р3ч 6 ай бұрын

Usually you should to incubate the membrane with bloaking solution during 1 hour. Then you should wash 3 times and incubate with primary Ab diluted in 5% milk PBS overnight. Then you schould wash 3 times and incubate with secondary Ab diluted in 5% milk PBS during 1 hour. Wash 3 times and make a picture.