FISH - Fluorescent In Situ Hybridization

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Henrik's Lab

Күн бұрын

Пікірлер: 123

@henrikslab 4 жыл бұрын

Which topics should be next? Please make suggestions here:

@harikabharadwaj98 3 жыл бұрын

DNA fingerprinting

@nbijetadevi1719 3 жыл бұрын

Microarray

@philippphilipp9832 3 жыл бұрын

Bacteriophage typing method

@darshanhegde7717 3 жыл бұрын

Karyotype versus FISH versus microarray versus targeted exome vs clinical exome

@shukuraopeyemi6670 2 жыл бұрын

Qq% 1%q@a1@100

@gabrielanunes146 Жыл бұрын

English is my second language and the way you talk very slow was just amazing for me, because I'm studying about FISH in my university in Brazil and I'm so proud of me to studying in English. By the way I have a test today wish me luck!

@mariociencia12 3 жыл бұрын

This is the best video about FISH that I saw on KZbin!

@cfuenza4106 2 жыл бұрын

Extremely awesome and relevant to the preimplantational genetic testing environment. Well done, clearly explained!

@Augetie 2 жыл бұрын

This helped me so much thank you for explaining in such a calm voice and tempo

@Augetie Жыл бұрын

@Mixkopf 38 it helped me lmao

@siyabendunus6443 4 жыл бұрын

Thank u. Nice german accent ;-)

@thetrollpatrol8799 Жыл бұрын

Why the wink

@niels1318 8 ай бұрын

@@thetrollpatrol8799 ;-)

@Vagolyk Жыл бұрын

Never thought this is how fish are made.

@utrlohan 5 жыл бұрын

Excellent work, thank you very much for your time and effort.

@alaechda9056 3 жыл бұрын

An exemple of how to design a probe for a specific gene will be nice

@telugufunnymoji5564 Жыл бұрын

How the deletion site is known . And what confirms that probe is bound like how it gives signal after binding to dna

@耿显 5 жыл бұрын

really clear and helpful....solved my problem about why we used small DNA fragments ,thanks a lot

@RahulKumar-mm5vm 2 жыл бұрын

I have a question regarding dna sequence using FISH. "Is it possible to identify a particular gene sequence (for example - Amel Y) using FISH if there is lot of depurination (loss of adenine , guanine) in interested gene sequence ?"

@doodoobearlove 4 жыл бұрын

Thank you totally clear my confusion! and right to the points!

@deniseoliver-stergiou7842 5 жыл бұрын

Wonderful easy to understand video! Thanks Henrik!

@lilbits661 2 жыл бұрын

Crazy German scientist over here. Thanks tho, it was very helpful!

@عزالدينالشيخسليمان 3 жыл бұрын

Nice explanation, You made the concept easy and digestible, thanks

@hollyashton7073 5 жыл бұрын

Very helpful! have you done one of CISH?

@deivibarci2093 3 жыл бұрын

Thanks a lot :))) You just saved me 3 hours 🌟🌟 Keep up the good work !!

@vlr003 4 ай бұрын

So helpful and clear, thanks!

@anusharamdurga6943 Жыл бұрын

Really Thank u so much sir for this video ☺️ it helped me a lot to do my seminar ....God bless you 🙏

@nmz61 Жыл бұрын

Thanks, that was easy to follow and understand.

@ruanfamilytv9658 4 жыл бұрын

2 Quick questions 1) how can the ligase seal the fluorescent nucleotides. They need to be bound first right? So my question is how do these labelled nucleotide bind? DNA polymerase will just randomly come along? 2) if i do the labelling before I amplify, how will the PCR be able to copy the fluorescent dntp? thank you

@Pearlblack6387 8 ай бұрын

in my opinion, ligase has some recognition site that recognizes the specific sequences and then it binds and causes ligation. DNA polymerase also has some specific sites that recognize first and then do polymerization. is this correct?

@priyasaha183 5 жыл бұрын

This video is very helpful to understand FISH easily

@rosette_renah Жыл бұрын

This was soooo helpful,,thank you

@meeromeer8812 Жыл бұрын

Thanks. I need to know how to figure out the used probes! For example: we have thousands of syndromes, do i have to make probes for all of them (especially if I have no idea about symptoms)?

@erkegirl Жыл бұрын

This video was real good!

@englishspoken8168 Жыл бұрын

Cell fixation Adding probe Denaturation Hybridisations

@Swati.ss567 4 жыл бұрын

Very clear n concise... Thanks a lot really

@lexa5950 3 жыл бұрын

This video was so helpful, thank you for your effort

@anirudhmy4528 5 жыл бұрын

Wow man very nicely done It was very helpful for me Thank a lot.

@henrikslab 5 жыл бұрын

anirudh my thank YOU for watching it and the feedback!

@santyadel6323 Жыл бұрын

That was very helpful, thank you

@kui635 3 жыл бұрын

Kurz und knackig, danke!

@franciafenovavy6608 7 ай бұрын

After denaturation, why will the target chromosome will hybridized with the probe instead of rebinding to its original strand?

@rosedeleema4217 3 жыл бұрын

Warm greetings. The short video is very helpful . But how to identify the specific complementary site in a chromosome . Or how do we know to prepare the complementary probe , on what idea this can be produced? If possible kindly send the answers. Thank you. Dr. Rise de leema .

@henrikslab 3 жыл бұрын

Usually you know the sequence of the complementary site since it is a gene you can look up in genome databases! Best Henrik

@dr.qaisarjan2440 3 жыл бұрын

Greatly well explained

@MinhLe-nw2zz 3 жыл бұрын

You try to give the video more brightness it will be great if you do

@taongamvula3313 3 жыл бұрын

Where is the DNA that the probe originates come from?

@henrikslab 3 жыл бұрын

The DNA probes for FISH can be ordered by companies which will synthesize them. Is that what you mean?

@trivapatel1915 3 жыл бұрын

Helped a lot thank you so much☺️

@meeromeer8812 Жыл бұрын

Thanks. Is it possible to tell which test do I have to do when I'm facing a syndrome?

@henrikslab Жыл бұрын

I would ask that a medical doctor!

@riamirto5002 2 жыл бұрын

Thank you! Really helpful!

@zglrd8938 4 жыл бұрын

Does interphasic fish allow us to detect both anuploidie and microdeletions or just anuploidie?

@medicaleducation8978 2 жыл бұрын

some time it gives false negative results because some time probe are not properly designed and sometime there is change in annealing temperature ? Am I right sir or any other reason of false negative result ?

@wuming_yd 4 жыл бұрын

do you heat the cells/tissue up to 95 C? will the cells/tissue be destroied by such a high temperature?

@dortartakovsky7123 5 жыл бұрын

How you can amplify the flourocent probe by PCR? it wouldn't increase the amount of the probe which is tagged

@thaliahurtadozegarra8516 3 жыл бұрын

thank you very much for this video!!!!,I understand all

@sangeethap5197 2 жыл бұрын

Useful sir 👏

@chocoberry434 20 күн бұрын

thank you so muchh for the explanation!!!

@tanjiawen7467 5 жыл бұрын

very detail and clear. thanks a lot

@mohammedal-hammadi5085 4 жыл бұрын

It's so helpful and clear video, thank you so much really

@mithratpmithra Ай бұрын

Is this a technique in genome mapping?...

@henrikslab Ай бұрын

One of many, yes

@Bror円 3 жыл бұрын

This is great!

@anisa7c 4 жыл бұрын

how to make sure that the probe is fully hybridized not the complimentary DNA ? thanks :)

@henrikslab 4 жыл бұрын

First of all: Good question! My answer is based on this paper: www.sciencedirect.com/science/article/pii/S259000721830008X If you make sure that the concentration of the probe is way higher than the concentration of the target dna (e.g. 10000 probes per dna strand) it should be way more likely that one of these probes bind after denaturation compared with the single sister strand of the dna Hope you could understand my explanation!

@ravioli6301 3 жыл бұрын

Is it correct that a ARRAY CGH is kinda a reversed FISH? U should def do a video about micro array especially the array CGH as it is also used for chromosomal DNA deficts :)

@lexc8714 3 жыл бұрын

So FISH can help in karotyping too?

@henrikslab 3 жыл бұрын

Yes

@kubranuraydn5036 5 жыл бұрын

very good video.

@Meowmeows24 3 жыл бұрын

What is the principal and the concept of the FISH technique ?

@henrikslab 3 жыл бұрын

It is to detect specific sequences on the patients chromosome (which are altered in disease). With FISH we make this sequence of interest visable using a "fluorescent probe".. this labels the sequence of interest

@Meowmeows24 3 жыл бұрын

@@henrikslab u help me , thank you SM😣🤍🤍🤍

@xaviasturm7248 9 ай бұрын

Gibt es auch ein Video auf deutsch ?

@zoew7872 9 ай бұрын

Can FISH detect mosaicism in an adult?

@siniorashani 3 жыл бұрын

Thanks very much ❤

@sonalimali8160 5 жыл бұрын

Very nice for understanding thank you

@ameliac504 3 жыл бұрын

THANKS! NEEDED FOR A PAPER

@zaysanatomy 4 жыл бұрын

So cool! Thank you!

@daenalund1613 4 жыл бұрын

Very helpful thank you so much!

@sadahauch910 5 жыл бұрын

Is Nick translation And FISH hybridization is same

@henrikslab 5 жыл бұрын

That is a good question, but here is the answer: So nick translation is just the process of getting your labelled probe. With this probe you can do whole process of hybridization then (FISHybridization).

@fabianperson 4 жыл бұрын

Nice accent man!

@englishspoken8168 Жыл бұрын

Fixation of cell et formaldehyde

@priyankaburange5832 Жыл бұрын

Thank youu !!

@sapthakathilakarathne242 3 жыл бұрын

thank you !!

@manishjadonrajput3095 4 жыл бұрын

Thank sir explain mutations.types like this.

@arnotrihalder1237 4 жыл бұрын

very helpful

@jaafar2562 4 жыл бұрын

Did anybody learn this in grade 12? because in lebanon we do .

@sylvia_forest 3 жыл бұрын

Yes I do. I'm learning this as a new chapter.

@jaafar2562 3 жыл бұрын

@@sylvia_forest ah ok thx

@idrisbagaruwagwarzo4363 2 жыл бұрын

I really do appreciate you Dr Igudia youtube,your commitment towards saving human lives is steadfast ,all the knowledge I got from you and,the help with the herbal meds, I was recently tested negative of Hepatitis B infection,I’m so happy thanks doc