Basics of flow cytometry, Part I: Gating and data analysis

Рет қаралды 237,092

Thermo Fisher Scientific

Күн бұрын

Пікірлер: 26

@adnan.q.753 5 жыл бұрын

Extremely informative webinar for beginners. Highly recommended.

@veeraji18 7 жыл бұрын

A very nice presentation explaining in simple language

@alyssabiondo2930 2 жыл бұрын

Such a fantastic webinar! Thank you!

@siddhidesai6532 6 жыл бұрын

wow, very informative and useful. thank you and keep uploading more.

@danieloulhint7914 2 жыл бұрын

Thank you so much for this informative webinar. I’ve learned a lot. Kudos

@thermofisher 2 жыл бұрын

Glad you liked the webinar, Daniel. Stay tuned for more.

@rangeo8783 3 жыл бұрын

Can we apply two different lazers (e.g., FITC and PE) at the same time to excite cells, and then detect and sort only cells that are exicted by both lazers, and get data from computer? This would be the same effect by Image J. (e.g. Getting FITC and PE images, respectively from fluorescence microscope and then merge them, which generates yellow pseudo color)

@thermofisher 3 жыл бұрын

Hi Range. Thank you for your question. Please contact our technical support team at thermofisher.com/askaquestion for additional information.

@Lokinenivenugopalrao 4 жыл бұрын

EXCELLENT....VERY INFORMATIVE

@thermofisher 4 жыл бұрын

Thank you! I'm glad you think so.

@khaliddar6139 5 жыл бұрын

Where can we find the other two lectures which were mentioned in the beginning of this lecture

@thermofisher 5 жыл бұрын

Thanks for watching and thanks for your question. You can find Flow Cytometry, Fluorescence, and Imaging Basics in our Molecular Probes School of Fluorescence - www.thermofisher.com/us/en/home/life-science/cell-analysis/cell-analysis-learning-center/molecular-probes-school-of-fluorescence.html

@ganglion0156 6 жыл бұрын

where we can get the power point to be able to read it in our hands and take notes on them?

@thermofisher 6 жыл бұрын

We contacted the team that created the deck, if it is still available, we will reach out to you to let you know how you can get a copy of it. Thanks for the request.

@elleb9526 4 жыл бұрын

why can histograms be used to map flow cytometry data?

@thermofisher 4 жыл бұрын

Hi Elle. Thanks for your question. Histograms are used as a way to look at a “shift” in a single channel (antibody). They’re not as informative as a scatter plot, where you would be able to look at he overlap/co-indicence between two different antibodies. For additional technical support, please contact us at thermofisher.com/askaquestion. Thank you!

@chieduepiphany9049 3 жыл бұрын

When is the next webinar going to take place

@thermofisher 3 жыл бұрын

Hi Chiedu, if you're looking for more videos or webinars on flow cytometry, we have a whole page full of them at the link below: www.thermofisher.com/us/en/home/life-science/cell-analysis/flow-cytometry/flow-cytometry-learning-center/flow-cytometry-resource-library/flow-cytometry-educational-videos-webinars.html

@fakeprincessII 7 жыл бұрын

The answer to question #1 fluorescence emission is always longer than excitation should be false. In cases of multi-photon, energy upconversion for example, excitation wavelength is longer than emission. I guess those 4% people answered correctly are those from physics or photonics or laser application background like myself :)

@toumperezh 7 жыл бұрын

Of course... but this video assumed a regular "single photon" laser excitation behavior. And even in this very context, if you have a closer look to the different spectra of emission of your fluorochromes, you will see that some photons do have a shorter emission wavelength than the laser used to excite them... typically FITC photons below 488nm... In reality, these photons exist in a "pre-excited state" before they receive the energy (h.v) from the laser. You can read Shapiro to know more about it.

@akshayd211 5 жыл бұрын

@@toumperezh Good stuff all round. Thanks!