This lady... well she changed the course of life on this earth. Not saying it’s good, nor bad, although the potential for both is of a very very high order.

I've listened to the Jennifer Douda audiobook on how CRISPR was recognized and developed. This short video was very informative seeing a top-down overview of the technology, what it is capable of and where the technology may be heading.

God bless Jennifer Doudna and all her colleagues and collaborators. Your work is truly amazing 🙏

I have met her in one of the international conferences, pre covid times.

What are the terms 'CRISPR' and 'cas' abbreviations for? CRISPR stands for 'Clustered regularly-interspaced short palindromic repeats' and cas stands for' 'CRISPR-associated'. What were the 2 main genomic elements of CRISPR first identified in E.coli? 1. The palindromic repeats, which are 20-40 nt in length 2. 'Spacer DNA' found between the repeats, all of which have unique sequences Which genomic locus are cas proteins transcribed from? The cas operon. What are the 3 genes that are found in the cas operon and what are their function? 1. cas1 and cas2: required for the acquisition of new 'spacer DNA' into the CRISPR system upon viral infection 2. cas9: the main effector enzyme that facilitates destruction of invading dsDNA through double-strand breaks What are CRISPR RNA (crRNA) and tracer RNA (tracrRNA)? 1. crRNA is the 'spacer DNA' derived from invading sequences that is integrated into the CRISPR system in the host genome (upstream of a palindromic repeat) 2. tracrRNA is a transcript that binds to crRNA and facilitates its association with cas9 What are the 2 regions of crRNA that aid in the destruction of invading nucleic acids? 1. The crRNA 5' sequence is derived from the invading nucleic acid and guides cas9 to the target DNA sequence 2. The crRNA 3' sequence (derived from the palindromic repeat) base pairs with the 5' region of tracrRNA, facilitating interaction with cas9 How was the CRISPR-cas system simplified for use in molecular biology? The crRNA and tracrRNA were combined into a single RNA known as a 'single guide RNA' (sgRNA). How can knockouts be generated using the CRISPR-cas system? Using a guide strand with a 5' region with complementarity to a gene and a 3' region that mimics the tracrRNA allows targeting of the cas9 enzyme to the desired locus and cleavage of the target transcript. This produces double-strand breaks in gDNA that are repaired, leaving indels that render the gene non-functional. How can knockins be generated using the CRISPR-cas system? Co-transfection with a targeting vector allows for homologous recombination to occur immediately after dsDNA cleavage by cas9. Have CRISPR-generated knockouts been demonstrated in the brain in vivo? Yes. What is the basis of the technique that uses CRISPR-cas to transcriptionally regulated a gene (rather than knock it in or out)? A non-functional varient of the cas9 enzyme - 'dcas9' is used. In this technique, the guide strand is modified to contain an MS2 sequence, which recognises and binds to the MS2 coat protein. Proteins which contain this 'coat' are then recruited to the genomic locus by the dcas9. What are the 4 types of protein that could be recruited to specific loci using dcas9 and MS2-containing guide strands? 1. Coactivator proteins (e.g. NCoA1) 2. Corepressor proteins (e.g. NCoR1) 3. Epigenetic modifying enzymes (e.g. CBP) 4. Transcription factors (e.g. CREB) How is the CRISPR-cas9 system used in vitro? A plasmids containing the cas9 gene and a plasmid containing the sgRNA are transfected into an appropriate cell type

It is an amazing lecture. I learnt a lot. Many thanks for sharing the video.

Other than amazing, what else? Happy to witness this amazing invention in my lifetime.

Wonderful lecture. Thank you for sharing it.

It's just woow congratulations prof Jennifer Doudna

A very important discovery that strongly impacts humanity, both for good and for bad, depends on us.

Thank you so much Dr from Egypt

This was just perfect… I just wonder why the pointer was not available 😢

I was saddened that the camera was focused on her and NOT the slide her pointer was referencing. This tech is advancing quickly and could become dangerous in the wrong hands. She should share a Noble prize for this incredible work.

Okay so after she won noble prize for this now KZbin is recommending each and every videos of her Oh my am learning this thing straight from her Wow thanks YT

Thanks for sharing! It is a very helpful lecture! Was hoping to find the associated technologies aspect but the fundaments answered a lot of questions already.

Excellent presentation, great respect and admiration. I want to learn more and more.

Really interesting and helpful talk to understand CRISPR technology, thank you!

Well defined CRISPR at 4:03 up to 5:05 Thanks 😊 alot

seeing how the technology is improving... making the future more and more exciting,

Welcome to everyone who's here after Dr. Doudna's Nobel Prize!

Fascinating Stuff. It's too bad we can't see what she is pointing at during her presentation

Congrats to Professor Doudna on her Nobel Prize. Is a copy of this excellent slide presentation available?

Next Nobel laureate

Good presentation, thank you

Thank you Prof

thank u for sharing, it very helpfull for me.

very useful ,thank you.

You observed that the CRISPR knock-out of protein X either promotes or represses RNA polymerase II transcription, depending on the gene. Which experiments would you carry out to reveal the mechanism for this differential activity?

Wondering a very fundamental question. Do all bacteria have this system? and, if so, does mitochondria or archaebacteria once had a similar system too? According to the hypothesis of the endosymbiont, most of mitochondrially encoded genes moved -over time- to the nucleus. Just a speculation whether early eukaryotic lineages may had used variations to this system to evolve complex genomes. This was a very nice talk. Thanks for posting.

Congratulations! Love and respect!

I suppose it is a very , very hard work!

Exellent ! What I don't understand is in what way pieces of incoming phage (or plasmid) DNA are cut out from the phage chromosome (by bacterial restriction system ?) and integrated into the CRISPER system (and also in what way) and why, at least what we are presented, these fragments are always of the same size?

Just seen this young lady being interviewed on BBC's Hard Talk.

Shes a genius god

What happens with methylation and histones, does cas9 only affect genes that are readily readable? I guess anyway that should be fine for most uses.

I would like to find out more about how the repeat palindrome folds into a hairpin, what tracRNA actually is and how it connects to that, how the whole chimera comes together, and how a piece of replacement host DNA is tacked on ??? ... The Professor is an awesome progenitor of one of the new century's most greatest technological advances, btw. - Can't wait till we have free-floating climate change eating bacteria.

A year later, we know know!

I wept when she won the Nobel even though I personally don't know her. She changed the future of science.

Why does cas9 not recognize nor cleave the bacterial DNA itself? I mean, if the bacterial genome has the viral sequence (the spacer), would not be possible that the cas9 cleave its own bacterial genome? I think that the answer has something to do with the PAM sequences which from what I could get are only present in the viral DNA but not in the integrated spacers within the CRISPR loci. However, I am not a hundred percent sure if this alone explains why the cas9 does not cleave its own DNA at these CRISPR loci. In fact, the probability of having a NGG nearby the spacer does not seems to be too low, unless there were some kind of negative selection.

My favorite scientist

Thanks a lot

Do you know where I can find these diagrams? These look very useful, I haven't been able to find such diagrams elsewhere.

Thanks

Is there a limit to the number of repeats, and by extension, a limit to the number of RNA/protein complexes that can be formed?

This was 4 years ago. How close are we to starting to knocking out genetic treatments for genetic diseases?

Can you try writing Doudna without writing DNA?

Why is it necessary for the barteria to have this system if it can recognize and remove viral DNA and neutralize it on initial infection ?

What i don't understand is how dosen't this system also cut out the viral DNA already integrated in the bacteria's genome (flanked by CRISPR) and thus inactivating the bacteria's response to futre similar viral infections

would please one of you guys tell me where is Natural CRISPR RNA and Tracer RNA at 14:29....cant get it

Thanks for sharing. Are there any lectures on non biological lipids?

Instead of focusing on her you could have shown the actual screen so we could see where she is pointing?😅

Do van der wal energies guide Or. is it all resonate energy

This is Wonderful. Great advancement. I also plan to buy stock in Crispr Stock Company.

Very inspiring.

Thank you! Interesting!

Congrats Jennifer

Welcome to the machine.

Is this the technology used to make our current Covid vaccines?

I wonder when it dawned on Jennifer Doudna that she should Do-DNA. I bet she was led by her surname to her science. ❤️👍🏻

When your surname is DNA it is fair.

they are expermenting this on me i am a target of this

She says in the wild, which we now know, are lab made with wild spike proteins

I am sorry ! I just learned about cas 1 and 2 and protospacer. However, dr. Doudna should have mentioned them at the very beginning of the otherwise great lecture.

Eventually it'll be a Bioshock situation.

The moving pointer is not Visible If it's visible then so beneficial to Us

Why did she get the prize for Chemistry rather than molecular biology?

Her name ends with DNA

How could I join this kind of presentation?

wonderful work, pity that there are people both for the search for good as you, as for the search for evil, sar cov virus was great target of this discussion of super virus families manufactured in laboratories, but all evolution is very welcome evolved congratulations. Viva la vida

Now know!

👏🏿👏🏿👏🏿

Dr Doudnas is a possibility that super research to be used to inactive coronavirus?.

I'm curious how these future generations of perfect humans will treat us, the inferiors... As we treat nature, animals, or just other humans because they are different?

¿Conoces esta verdad? 1. Las nubes del cielo de todo el mundo son bajando a la tierra cada día más. 2. El sol y la luna en el cielo son superlunas y super sol todos los dias. 3. Si observa de cerca el amanecer y el atardecer, puedes ver el cielo rosado. 4. Los componentes químicos de Chemtrail se pulverizan como loco en el cielo de todo el mundo. 5. Si miras de cerca la luna ahora, la luna está girando.

Cant we use this crispr technique to infect those bacterial genomes with covid19 virus to find the resistance gene incorporated in bacterial genome against it..and then test that in humans?

Very persuading woman

What are 'bp' and 'nt'. i see them used in articles on crispr and in this video as well. I'm doing a research assignment on crispr technology, someone pls answer asap.

Hopefully with the new administration in the US, funding for science research is boosted and not cut further.

cant hear questions

41:50

Why CRISPER CAS9 genome editing technology get Nobel Prize in chemistry field?? Why not physiology/ medicine field?? This topic is biological topic.. then why Nobel in Chemistry? ❤️❤️❤️from India.

Covid-19?

I wish I could understand lol

Can we use this to fight the coronavirus if we were to inserting a copy of the messenger mRNA into a similar vascular or monocytes similar to the virus package lysosome or monocytes? The messenger mRNA of installing two stopped codons on both ends of the messenger mRNA ,so when the virus enters the cell RNA from the virus is then match to the messenger RNA that is waiting for the mRNA for the binding once the messenger mRNA It is now considered to be a safe proteins ,and RNA molecule and once it is duplicated with the chaperones through the nuclear tides being tied together forming new inactivate DNA strand that will be not be able to be used within the cell.

She describes intelligent genetic design.

Ok so you basically very carefully giving a lecture on how the Chinese Caucasian Arab and y'all was created I've done research and there's alot of missing information and wholes and you very much aware of the fact n using deceiving words like real quickly and and not going into details and using cartoon to make mockery so one won't think nothing of it

The American taxpayer is one source of funding. Rather than compulsory means, extracting from many who are struggling to make ends meet, why not collaborate with the super rich who happen to be personally interested in such research and are unquestionably able to do so without subtracting so much as a crumb from their own table - someone like Bill Gates?

Yea, like Einstein she wanted to make the world better. But I think this technique will do more harm than good.

The cruel sardine markedly warn because hexagon dentsply attack unlike a noxious raft. giant, faint fair milkshake

Made in the image of God. Blessings ! Jesus will return are you ready? XO Then Jesus spoke to them again, saying, “I am the light of the world. He who follows Me shall not walk in darkness, but have the light of life.” (John 8:12)

If youre looking for a way to understand crisps cas9 without no prior knowledge then this is a bad presentation for you and you should go back to reading. So sorry to say this because i don't want it to be. Maybe her audience has taken a few university courses and thats why she doesn't break it down as much as i would like. Dammit its hard to understand geniuses without reference books.

Dr DO-YOU-DNA coincidence enough?

not much help at all when she points the pointer into the middle distance, rather than showing the target, viz. the diagram

PROTECT HER AT ALL COSTS!!!!!