Hello, nice to see your channel! Each episode is very helpful. Thank you for sharing your experience.

Great video and explanation! Helped me prep for a job interview doing a lot of flow and this was just what I needed.

Thanks for the great work.

Great video and great explanation

The fact that this sounds like it is being taught to a 12 year old. I love it.lol A great teacher. I actually understand the WHYs so clearly now. Thanks.

Thank you so much for these great videos and clear explanations.

You’re the best, Aja❤ love your videos and I use them as a resource for introducing people to flow. Yours in Flow, FlowJoe Guy

Excellent verbal skills. It is engaging with flawless progression throught the entire video. thank you so much!!!

In the top left corner of the FlowJo compensation window there is an optional "Spectral" checkbox. How is that different from what you describe in this video?

Hi Aja, great thanks for those clear explanation. My name is Yoo Sun Kim and I'm a postdoc working at NCI(NIH/US). I just started using multicolors flow which is so exciting, and I enjoy learning and using the machine. Would you mind if I ask you a couple of questions regarding compensation controls? I'm looking at tumor infiltrated immune cells populations. 1. Would it be ok if the compensation controls experimental samples are different cells (sources) ? For examples, I use syngeneic mouse splenocyte for compensation controls because cells are positive for most of markers and I get lot of cells. The experimental samples I would like to run is tumor infiltrated immune cells. 2. If the answer from above is yes, would it be acceptable if I use only one marker (such as CD45 which gives strong signal) for all the different parameters? I'm asking because I realized that if I have to compensate markers for active T cells, such asCD69, I had to stimulate splenocyte prior the staining. So I justthought it might be the easiest way if I could use just one marker for all the different parameters. But I was not sure the it makes sense. For example, when I do CD3+ (561nm, YG586) single stain control from splenocyte, I had to decrease the laser voltage pretty lot to see a nice separation, do you think it would it be the same even though I use CD45+ marker for YG586 color compensation? ( I can get the answer if I do it myself :), yes I'm going to order CD45 YG586 antibody..and I'll get back to you when I get the results! but still I just would like to know your thoughts!) Those were two questions I had. Thanks for reading it, look forward to hearing from you. Again, thanks for those fantastic videos! Best, Yoo Sun

Thank you for the great explanation. Can you please make a video showing the actual procedure of compensation on your computer? What if you do not use the Wizard but the table? Do you separate the steps, one compensation for the single stains, and another one for the beads? Thank you again.

Good teacher! Very helpful. May I reuse my compensation if I use the same beads for each single color control? Thank you!

Hello- I have a question. What is the best way to correct “over” compensated samples? I have an issue with BV750 and AF647.

Hi Aja, I encountered a tough problem on mcherry spillover with other dyes. Here is my case. I started a new experiment to use mcherry labeled lentivirus to edit cell membrane protein X on the cell for knockdown. I detected the mcherry population for viral titration as well as the target protein X expression staining by X-biotin + streptavidin-PE combination due to the low expression of protein X. When I run Fortessa machine to create my compensation for PE(beads), mcherry+ (a mix of transduced cells), unstain (looks like cells are better than beads from this experience). PE was easy to show a narrow peak for positive, however, mcherry was hard to present a peak for positive, which require unstain cells for me to decide a gate to show positive from negative. Even in this careful operation, the machine also warns 200% spillover of PE on mcherry or 200% spillover of mcherry on PE (Sorry, I forget the exact description). How should I do to save this spillover problem? Here is my thinking. First, I will try another dye, such as streptavidin-BUV395, which is not spilled over with mcherry , due to different lasers to excite them individually. Second, if I didn't change fluorochrome, I will try spectral flow cytometry, like aurora. Could you give me a comment or other suggestions? Thanks!

Amazing video, Dr., the link to Flow Post-its from MSKCC is no longer available :((, do you have another link to it?

hi, I didn't understand what you mean by cowboying compensation, could you explain? :

Why do compensation matrices change so dramatically over even a single day?

what's with the intro