Awesome awesome . I was reading the textbook and not getting it . But after watching it whole stuff is clear . Thank you much ❤️ for this video.

The most useful video on filtration columns!

I absolutely love this video! Thank you!

Very clear demonstration. Thank you

This is a very useful explanation. Thanks.

Hi, this is a very helpful video. I had a question. What is the best way to tell which fraction contains the protein if the everything we are dealing with is colorless?

If anything catches on fire at the lab tonight, i will blame you cause i will follow your method.

Hello Dear 👋 Thank you for good tutorials actually I have one question is there any different between Gel Filtration LH-20 and HiTrap Desalting because both packed with G-25 and for purification secondary metabolite I need LH-20 but HiTrap more convinced I will appreciate if you give me good answers because I am working on unknown components

Thank you so much, I really did understand. Please is there another video for calculations as to help one plot a graph? If there is one, I will be waiting. Thank you once again

Such a helpful demonstration. Could u help me with few queries.. Does the flow rate of buffer hampers the separation of protein? What should be the flow rate and what amount of protein can we load into the resin?

How do you know when to swap the test tube drain caches?

Very nice demonstration 👏❤️..Thank you🙏

I take plant extract, i want different component of plant extract, which method is useful and accurate to separate plant extract component?

Excellent video! Thank you!

Well explained Great 👍👍

Thanks! This is incredibly helpful

Very nice video presentation!

One of the best videos regarding size exclusion chromatography. I have some questions if you do not mind. I have bought Superdex 75 resin. If am not mistaken, I should pour the resin and let it for one or two days in a falcon tube eg to calculate the slurry (if I pour 10 mL of the resin and the new measurement is 5.5 mL it would be 55% of slurry). And then add this slurry into the column. My question is if I understood that correctly. Also, my column can host up to 16 mL, what is the preferred bed height to apply? I saw you have written about a 1:12 ratio of volumes. Finally, after packing a column, how many times can it be reused? Thank you in advance

Very nice demonstration..Thank you.

How to make blue dextran.. We should dissolve into distilled water or in phosphate buffer plz tell me

very nicely explained thank u so much!!!

Good day, sir. Can I ask what kind pf column is that? Can I use the conventional glass open column (similar to those used for silica gel)?

Hi, I used sephadex G25 and packed the column similar to what's shown in the video. However, fluorescein doesn't retain as in the video but travels right though. Do you apply pressure in packing the column?

would the steps be the same (+ the buffer used) for Sephadex LH20?

what solvent did you put the 9 grams of sepahdex in? Was it water or alcohol?

How much volume buffer did you use for the 9 g?

May l know the concentration of both the dyes .

Thank you, you made my day 😊😊

This was helpful, as there was no protocol on the GE website, you mention that 800 uL was a bit too much for this column, what volume of column per volume of sample is the limit?

What is the column you are using? Thank you.

Thanks for your nice video. What is the name of the empty column you used?

Thank you so much for this 😄😄😄

I am using Sephadex LH20 to separate and purify proanthocyanidins from wine. Methanol is the solvent. Bed volume 290 ml, with 4ml/g of dry material used for given solvent. How big should my sample be without causing poor seperation/resolution? Thanks!

Thank you this is a huge help! How much buffer did you swell 9g of sephadex in, in the beaker?

Thank you so much for making this video

Why does the larger molecule move faster?

Can I use distilled water in replace of tris buffer?

Hello. My lab manual says to "Pour a column (Sephadex G-75 slurry) so that the bed is about 13 cm in height. Equilibrate the column in the elution buffer." Would equilibrating the column be what you did from 1:45 to 2:13?

thanks for tutorial!

s it possible to separate the sizes of DNA?

Can anyone help me to know: What's the scientific name of this type of tubes used for this purpose? Thanks

Can anybody recommend a process to purify an Oligonucleotide Mix in RNase Free Water. These oligos were only standard desalted. The volumes vary from 250mL to 1400mL. thank you Spencer

thanks for your help

My gel (Sephadex G-100) keep running through out the columm. I dont know if it is the consistency or maybe the buffer I used to swell it up (sodium acetate 50mM pH 5,0 - the enzime Im looking to purify is well adapted to the this buffer) is not appropriate for it. Should I plug a small piece of cotton to the botton of my columm and then add the sephadex to avoid the gel to leak out?

Thank you!!!

Thank you!

How to extract ricin protein from this process??

Nicely explained

What kind of column is that?

amazing

Can you please guide me how I can purify a protein of mw 40kd using chromatography from a fermented broth.

This vid is very help, thank you so much!

thank you

Thankuuuu

What's the expiry date of the packed gel in the column?

what if you drink it?

What's name of buffer

Lovely

Thank you, :)

Neeru ma'am bought me here.

Thank you sooo muchhh❤️❤️❤️

Its very useful.

Nice

nice, it will help :)

dank goethe uni so viele views

Thank u sir

Biochem squad

useful

what was the buffer you used?

To many bubbles! But still a nice video ✌

sigma sephadex

wer ist hier wegen dem Biochemie Praktikum hahah?

Can you please guide me how can I purify a protein of MW 20-25 KDa using chromatography from a conjugation buffer