Agarose Gel Electrophoresis
ฝัง
- เผยแพร่เมื่อ 10 ต.ค. 2012
- For more information, visit www.bio-rad.com/yt/idea.
This video demonstrates how to load and run DNA samples on an agarose gel. Basic information about the charge of DNA and how it will run in an horizontal electrophoresis cell is explained.
www.bio-rad.com/evportal/desti...
We Are Bio-Rad Explorer.
Our Mission: Bio-Rad’s Explorer program provides easy access to engaging hands-on science learning experiences that spark interest in science and its influence on the world.
To do this we:
Provide high quality, relevant, learning experiences based on real world science
Empower educators with skills and confidence to deliver engaging, memorable lessons
Connect with Bio-Rad Explorer Online:
Website: www.bio-rad.com/en-us/education
Twitter: / bioradeducation
Pinterest: / bioradexplorer
LinkedIn: / 1613226
Facebook: / biorad
Instagram: @BioRadLabs
Snapchat: @BioRadLabs - วิทยาศาสตร์และเทคโนโลยี
Hop Barış hocamdan geldik buradayız
barış hoca da olmasa geleneksel eğitim metotlarına maruz kalmaya devam edeceğiz
ben de ordan geldim sdkfsdmögs
Ben de chhdj
barış hocam yolladı bizi buralara
o kim
@@noth3285 barış hoca biyoloji
Evetttt
Dr biyoloji
Ayn
barış hocam sağ olsun
EVET EVET!
Barış hocadan gelenler yazsın buraya yks savaşçısiyizzz
Barış Hoca'dan gelenler
BARIŞ HOCAM SAĞOLSUN BİZİ DENEYLERE ORTAK ETTİ
barış hocadan gelenler
Barış hocadan geldik.
Barış hocam da barış hocam
aşwldşlawdşşad
Barış hocamdan buraya transfer olduk
Barış hocadan gelenler ses verin 🤝
ben ben ben
ben dee 🤘
Kazandınız mıı
asla cevap vermezler...
@@YKS2006
barış hocadan geldim
Barış hocadan gelenlere sa
Barış Hocadan gelen arkadaşım sana da selam olsun
We brought the greetings of our valuable teacher Barış M. Kapan
DR Biyoloji den gelenler
Barıs hoca kalitesiyle buradayız
barış hocam sağ olsun deneyleri görebiliyoz
Barış Hocam'dan geldim.❤
How many student came from Dr biyology?
@DR.BİYOLOJİ HOCAMDAN SELAMLAR
Dr. Biyoloji 💐
Dr. Biyoloji Dı dım tı tıs 🥁
Barış hocam bir tane 😊😊
I just realized why I was doing this in lab because the instructor did not explain a thing! Thanks soo much! God bless 🙏🏻
Thankfully my instructor is a boss and covered all of this and used this to show the process, hope you get a better teacher next semester.
I'm interestingly interested in this
Barış Hocamda Barış Hocam
Barış Hoca sayesinde geldik
Barış hocam 🤟🤟
Barış hocamda barış hocammmmm
Dr Biyoloji🫡
Barış hocam gönderdi O7
Excellent description on GEL ELECTROPHORESIS...MANY THANKS FOR UPLOADING THIS LECTURE ❤️
Amazing...to see the DNA fragments...1. Smaller the fragment size ,the farther it moves. 2.Agarose is natural polymer extracted from Sea weeds. 3.Separated DNA fragments can be visualised after staining with ethidium bromide.
NCERT! 😂👌
Who the hell still uses ethidium bromide!??!? SMH...SYBR Safe has been around for like a couple of decades now...there's absolutely no need to keep using the HIGHLY carcinogenic EtBr...wow...
Came from "DR. BİYOLOJİ" chanel 🤙
1. siapkan sub sel mini
2. sejajarkan gel sehingga sumur paling dekat dengan elektrode negatif
3. tempatkan egl agarosa ke ruang gel
4. tambahkan buffer elektroforesis ke reservoir sampai reservoir tertutup buffer elektroforesis sedalam 2mm
5. tempatkan sampel sesuai urutan yang benar
6. tempatkan sampel ke dalam sumur dengan menggunakan mikropipet. jagalah pipet tetep tegak lurus terhadap lubang
7. pasang tutup ruang gel sesuai dengan elektrodanya (hitam ke hitam, merah ke merah)
8. sambungkan elektrode ke catu daya
9. nyalakan catu daya
10. atur tegangan konstan sebesar 100V
11. atur timer menjadi 60s
12. amati perubahan yang terjadi
Lovely, I'm interestingly interested in this.
I just finished running the three practicals now, on center for molecular bioscience and biotechnology lab in SCH
Hi can i ask you some questions maybe in the future for academic purposes only. thank you. is it okay if i can contact you through email?
Nomesh sir PW show this in class 😎😎 rewatching this video after class ❤❤
Thank you for this
So exciting, this!
Watching it during quarantine 😭😭😝
haha
Omg i passed that semester and still corona didn’t ended
@@sondos8928 hahahaha I’m doing it for mine right now
@@sondos8928 "ended"
im sorry quarantine was a year ago-? holy shit-
I'm coming from Barış hoca youtube chanel❤
How nostalgic. I did this as a practical exam when I was in college and completely ruined the agarose gel 😂😭😭. My prof got really mad.
Damn can't wait till I go to college...
What happened exactly? How does one ruin the agarose?
very informative . thanks a lot.
Thanks
What should we do if there more bubble in red electrode?
Please make a video on sample preparation also
Thank you so much. I learned lessons but i never applied and i am still scared 😅
thanks my dude
1:56 oh, that is so damn satisfying.
When he pippet sucked the entire sample I said fukkkk so perfect
for the blanck I use the leader + load dye. for samples of dna you need load dye + dna + enzime + enzime buffer, I am missing something?
Thank you.. Well explained
osmmm video! plzz upload more more dis kind of video so that it is to understand
very Informative
This is very nailed and good knowledge thanks 🙂
very well done video
instead of pushing the pipette all the way through when loading the wells, you could release pressure to suck the bubble back in. that way you avoid marked sample spilling out of the wells - not that it makes a huge difference, i just like to keep the buffer clean.
Or you could not push to the second stop
@@Ronnicus lol
For the bands to be visible…. No need for ethidium bromide and uv light exposure?
excellent videos
how I can label the product of gel electrophoresis by which program if my gel image was taken
by JPA please kindly for you recommend me thanks
I love it =) It's so interesting and beautiful at the same time =)
So are you :p
barış hocamdan geldikkk
This was awesome
Very informative.
Very cool video, well done!
Thank you so much!
Is fast blast DNA stain as good as ethidium bromide,i mean can it practically replace ethidium bromide,are there any hazzards concerned with this stain as it is with ethidium bromide
+Neelam Singh,
In our University Biochemistry lab today, we used SYBR safe DNA Gel Stain. It is less mutagenic than ethidium bromide, and can be used under blue light just like ethidium bromide.
I would feel much more comfortable buying this solution from Thermofisher Scientific. You can buy the solution here, as well as see the tests used to validate its efficiency on this page, as well. (Notice how the page is padlocked when you follow the link.)
www.thermofisher.com/us/en/home/life-science/dna-rna-purification-analysis/nucleic-acid-gel-electrophoresis/dna-stains/sybr-safe.html
What do we need the buffer for ?
really good
Very good information tq it is useful of my lesson .
Thank sir, I got it❤❤❤
Hello, any distributor of this instrumentation and consumable in Indonesia? Thank you
that was great thank you
Very understanding , thank you
That's my favourite experiment
I don’t need sybr dye for this step right?
Which dye do you use? And do you add the dye into the centrifuge?
Ethirium Bromide as the movement indicator and Bromopropanal as the blue dye.
Nomesh sir jindabad
Harika bi sey
Excellent thank you too much
Very Interesting 👍🙏
barış hocadan geldikk
Thank you!
thanks .. its good to learn the exact technique.
Thanks. It’s very clear
Good effort
thanks helpful
De
Please DO NOT stick your pipette tip in the well while loading,you might puncture it, not to mention the sample might hit the well and spurt outside the well.pour enough buffer so that your tip is immersed but is still right above the well and release sample slowly. The loading buffer in your sample, in this case the blue stuff, contains glycerol which is heavy and 'leads' your DNA safely in the well.
I do what I want
@@whatevervlogs9663 you can choose to learn or not. your call mate 🤷
Actually I'm curious to know how to load the sample.if I simply put the sample in the well doesn't it get mixed with buffer.or u directly put the sample inside the agarose??
@@srividhyanarayanan7337 your sample should already have buffer in it because you use the Loading Buffer LB I use a 1 microliter of 6x loading buffer (trisborate a couple of dyes and glycerol) and 5 microliters sample therefore your LB is diluted to 1x. If you are using 1x TBE or TAE the liquids in theory are close isotonically even though the actual samples vary. do not worry. the glycerol in your LB is heavy enough it will pull the sample into your well because gravity. Just practise a bit - put the tip above the well IN THE BUFFER and slowly release sample (no bubbles) you will see your sample-dye sink to the bottom of well. Maniatis protocols explain this nicely. Let me know if you need a recipe for LB .
@@papoutsothiki I don't think that's a thing, the pipette is supposed to puncture through the gel to allow the plasmid dna/ genomic dna to enter the electrophoresis casette
fantastic
Thank you! This helped a lot! But hey, where's ethidium bromide and UV rays? And bright orange bands of DNA?
Yes.. Atlast we visualize clear bands by uv rays .. They didn't mentioned it
very very good
what can be used as buffer solution except for tbe and tae?
Water
Why do we see more bubbles at the black electrode ?
Thanks
🙏thank you 🙏
When we did it we couldn't really find the wells and struggled for almost an hour and a half to find the wells.
Please how to prepare agarose gel and buffer to post the vedio
It's very important.thanks.
Tysm sir
gooood informations for less learn some choose and thanksyou
Thanks ❤
Its helpful ,thanks but please explain material reagents and their usage..