SDS-PAGE explained - Protein Separation Technique

Рет қаралды 189,818

3 жыл бұрын

Hey Friends,
SDS-PAGE (Sodium Dodecyl Sulfate PolyAcrylamide Gel Electrophoresis) is used to separate proteins in a sample according to their molecular weight.
SDS binds to linearised proteins and masks the native charge. 1.4 g SDS bind per 1g protein, so that all proteins have a nearly similar mass-to-charge ratio.
After an SDS-PAGE, the gel is frequently used for Western Blot analysis to confirm the presence of a specific protein of interest.
Western Blot:
• Western Blot / Protein...
Here is a helpful explanation on SDS-PAGE:
ruo.mbl.co.jp/bio/e/support/m...
Thanks & Bye
Henrik

Пікірлер: 70

@amrobay152 2 жыл бұрын

wow, after each video, i ask myself "why professors can not explain it that simply", thanks a lot!

@demaamro8750 2 жыл бұрын

Are we related? 👀

@nikpelekanou 11 ай бұрын

exactly that I'm Greek I study in Greek university and it s easier for me to learn all this in English than our notes that she gave us its not make sense she put so much useless details and they lost the mane subjects thanks for every one that really want to teach and not go to just do their job take the money and go

@talkbiology01 6 ай бұрын

Because they have to pass the time

@rahman1314 10 ай бұрын

at this point , i think the prof don't understand the process, if you can't explain it this simply as in this video, then at least give us link to videos that explains it better to make our life easier

@iguana1677 2 жыл бұрын

Clear & concise. Well-done!

@galaxyeyes1457 2 жыл бұрын

Thanks for making these nice videos. They’re very clear and the diagrams/animations are really helpful

@SaraMonicaLeonUlloa 11 ай бұрын

Excellent material! This is a great job explaining and illustrating the topic. Very clear information.

@wissammukaddam1393 2 жыл бұрын

What a brilliantly concise explanation, thank you.

@kimbokjoo6817 2 жыл бұрын

I watch all the ads for Henrik. He’s been very helpful.

@henrikslab 2 жыл бұрын

Ahahahaha

@dermdoc3637 7 ай бұрын

bro this video is so good and so easy to understand thanks a ton dude

@metarasouli 6 ай бұрын

Such a wow video should be appreciated. Thanks for sharing this video

@refad333 2 жыл бұрын

Very accurate and clear explanation. Thank you

@lotti7819 Жыл бұрын

thank you so much, you helped me a lot with my lab report!!

@Matt-tv5ww 2 жыл бұрын

this is the best SDS-Page explanation on the entire internet, thank you

@ahmetziyaaktas9179 10 ай бұрын

U explaining so clearly thank you 🙏

@jiinnyyk9483 Жыл бұрын

your video was so helpful!!! thank u very much❤

@graemelaubach3106 Жыл бұрын

You make the most informative and easy to understand videos. Thank you :D

@philbertnshimiyimana155 Жыл бұрын

I like this tutorial much. Very hepful in my current research project on p38 protein kinase

@razasyed575 11 ай бұрын

amazing video and explanation, thanks hoss

@aqsanadir153 2 жыл бұрын

You just made my day useful

@henrikslab 2 жыл бұрын

Well, that´s nice to hear!

@isadorah4969 4 ай бұрын

I want to become a teacher which explains clear and easy like u!!!

@bioscienceswithshahtareenswati 2 жыл бұрын

👏👏Wellstone. Well explained

@user-le1yx1bu8s 5 ай бұрын

Super nice video!!! ❤

@iidmukhtarjama9245 9 ай бұрын

Your videos are absolutely amazing Please I didn’t see video about southern and northern blotting

@3003wertpro Жыл бұрын

Perfect Video!

@fordmustang4945 2 жыл бұрын

Thank you very much you just save my marks for viva

@henrikslab 2 жыл бұрын

Amazing!

@omolemoratsoana4668 2 жыл бұрын

Thank you so much 🙏🏽

@sterlingteall3462 Жыл бұрын

Very well made video

@akhlasalarbi5690 Жыл бұрын

Wonderful ❤

@vivavampira249 2 жыл бұрын

thank you very much!

@storieswithmusab Жыл бұрын

Thank you professor

@ellios5734 2 жыл бұрын

thank you so much amazing

@bighooligan100 2 жыл бұрын

What site did you use to produce that sds image with the bands I’m doing my dissertation on cspg4 protein and have ran sds page for analysis and would like a neat version like yours on your animation as an image to my real life image

@henrikslab 2 жыл бұрын

Microsoft Powerpoint

@aliciacampelo5324 6 ай бұрын

thank you!

@ataraxie4086 4 ай бұрын

Danke!!!!

@amooooeba Ай бұрын

God bless u

@svitlanababych4051 Жыл бұрын

Can you turn on subtitles?

@soulboken4670 2 жыл бұрын

good shit

@salmaali-cf3od Жыл бұрын

thank uuu for the videoo

@biplabnayak315 Жыл бұрын

After watching this... i thought why my professor has to make every simple things present in a such complicated manner...why...

@henrikslab Жыл бұрын

In many cases, because they were never really taught how to teach...

@josefinesfilmtube 2 жыл бұрын

can you use this method to find protein protein interactions?

@henrikslab 2 жыл бұрын

This technique is part of another method that can be used for that: Immunoprecipitation... you direct an antibody against the protein of interest (want to find out the interaction partners of that protein)... you isolate this protein and everything that is binding to it. Then you can run SDS PAGE to see the size of the proteins you have pulled down with your target.

@josefinesfilmtube 2 жыл бұрын

@@henrikslab thank you so much for your explanation!

@laithibraheem7476 2 жыл бұрын

but why cant we use a normal gel elektrofores for it. why must the protien be unfolded

@henrikslab 2 жыл бұрын

If the proteins are unfolded it is difficult to sort them accoriding to their size (in kD)... Why? Because some proteins may folded like a tightly packed ball whereas others have a longer structure... to make that equal unfolding is important. Apart from that, the unfolding is essential to mask the charges (this would not be possible when they are tightly packed).

@IlanHirschfield Жыл бұрын

Very well-explained! Only comment/suggestion I have is that the negative terminal at the top is the anode, which is the negative terminal. The cathode is the positive terminal. The positive and negative terminals are labelled properly but the terms should be flipped in terms of their positions. Keep up the good wor!k!

@washuttleworth Жыл бұрын

This is the case for a galvanic cell it is reversed in electrophoresis, the positive pole is the anode. It is confusing but below is the explanation. In a galvanic cell, the anode is (-), and the focus is on pushing away electrons from the anode to supply power. In an electrolytic cell and gel electrophoresis, the anode is (+) and the focus is on attracting the negative ions in solution from inputted power.

@arathy592 3 жыл бұрын

Wht does buffer soln contain.?

@henrikslab 3 жыл бұрын

Usually, for SDS one uses the TRIS-GLYCIN BUFFER: It contains Tris, Glycin and SDS (0.1%)

@arathy592 3 жыл бұрын

@@henrikslab and u didnt mention about bromophenol blue..glycerol..gel preparation...or is there any another video?can u help me?

@mad.i.mp3 5 ай бұрын

min 1:48 i cannot understand what he says: having the equal _______ help please

@jasperpauli 3 ай бұрын

"the equal mass to charge ratio"

@presleymumba5995 10 ай бұрын

I love you ❤❤

@TheLa0la 10 ай бұрын

Du könntest ein bisschen an deinem deutschen Akzent arbeiten :P Aber super Video!!! vielen Dank!!

@user-lw7so7de6n Жыл бұрын

you need to adjust the content

@BossAwesome11 Жыл бұрын

Isn’t anode negative and Cathode positive

@ineskaineska8140 4 ай бұрын

لي جا من عند معماش يخبط جام 😂😂😂

@emirkaplan9844 6 ай бұрын

I've seen some buffoons that couldnt explain in 30 mins. But all bro neded was 4 mins

@karthikmatta509 3 жыл бұрын

Low Voice

@Th3Cryton 3 жыл бұрын

deutsches voiceover wäre auch nice :)

@ffynab2733 3 жыл бұрын

würde Sinn machen, es gibt nämlich kein vernünftiges Vid auf deutsch

@michaelafehringer3679 2 жыл бұрын

In der Wissenschaft sollte man aber schon Englisch können ^^

@kohlrabenschwanz 2 жыл бұрын

Sei doch froh dass du gleich bisschen scientific English lernst. Hilft auf jeden Fall wenn du mal vorhast papers zu lesen.