This is the most thorough HPLC series I found. Brilliant work. Thank you good person.

thanks for the hplc vids. in biotech program in dayton and you do a great job explaining everything.

Thanks for the effort in putting this material on youtube, I've been searching more of all of this topic and I don't find more clear material than this!! thanks a lot :-)

Thank you so much! You saved me and a great starter for my new PhD project!

Very impressive way of explaining materials. Loved that!

Thank you man for this hope you're doing well again thanks a lot.its overpwoered content

I really love how you explain all of this, its so clear and i could understand it easily, thank you so much for making this lecture 🙏☺️

Up to this episode, this series has been extremely insightful and helpful! I think this knowledge will help me very much in my upcoming job interview(s).

Thank you Sir. It was so practical for me🌸

thanks and can't wait for the next one!

Simply excellent way too much clarity in his lecture. You are Star.

I love your lectures! - A small tip: PLEASE start using a wacom tablet instead of a mouse for writing on the screen

I love your video. You make things so clear. Thank you!

Keep it coming , great stuff

These lectures help me out so much!! Thanks a lot!

😭❤️ thank you for the great job 💜💙💕

Thank you very much. Very helping to understand.

Thank you so much it is very helpful

Thank you so much for all these videos! it really helped me a lot in understanding and perhaps some troubleshooting on HPLC :)) maybe the next HPLC video could be somewhere around trouble shooting the result of the peaks? maybe on the shape of the peak, what is a good shape, what is a bad shape, what does it mean and what can we do to it. and maybe by then we can do some data analysis? :D thank you!!

thanks a lot i am waiting the coming videos.

I’ve been waiting for this haha

Thanks for this video, but I have one question at the time 43:13 of this video. you told that H2O/MeOH (in comparison to CH3CN/THF) has a higher Rt or longer spread. While in Revers Phase, the Stationary phase is Hydrophobic, and the more polar mobile phase should elute faster. Or I,m wrong? please explain a little more about this. Thanks a lot

Kindly, where is the link to the video that talks about HPLC columns ? thank you.

Hi this was a great lecture. Im curious though, if the peaks give the same retention time in the chromatogram for multiple analytes, how do you separate them and determine which analyte is which? Also does elution just mean how fast it will be detected by the detector? So a polar analyte will have a lower elution time?

Hi, Do you have any lectures about different types of columns? Analytical and preparative columns? Thanks

Thank you

And I paid over $1200 US dollars for a course over 27 years ago which didn't even touch HPLC , it was in the syllabus,, because the only Professor canceled the lab coursework..terrible to do that to eager mind at the time. I was sure to get my money back for the class.

thank you so much

Wow , thank you

Great

Okay so first, you'd play with the mobile phase. If that doesn't work change the colomn because of expenses?

Dear Sir, this is a help request, I have a question : is it true that more the elution power, less the retention time irrespective of the analyte? for instance I have a sample of Lactic Acid. I run HPLC using water as mobile phase and get retention time t1, I do the same but with acetonitrile as the mobile phase and get retention time t2, will t2 be < t1 ? Will t2< t1 be true irrespective of the sample ( say i use bezoic acid instead of lactic acid)

Bharat Mata ki Jai, ram ram, om namo shree Sairam namah shivay Narayan.

hi

Hplc not easier before this.

\Awesome upload! I believe you'd enjoy my content too. Keep up with the fantastic work! 💛💛

Thank you very much