Getting Started with Whole Genome Sequencing -

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Getting Started with Whole Genome Sequencing -

Рет қаралды 65,984

Күн бұрын

Want a deeper and more complete picture of the genome? Need to identify potential disease-causing variants? Studying a novel organism where no genome information is available?
Whole Genome Sequencing (WGS) can help you achieve all of this and more. Since the advent of Next Gen. Sequencing in 2008, Whole Genome Sequencing has been unlocking the mysteries of the genome with unprecedented resolution!
In this webinar, you'll get an introductory overview of how WGS works as well as key considerations to keep in mind when setting up your WGS experimental workflow. To end off the webinar, we'll also show you how to verify your plasmids using NGS!
You'll learn about:
• A brief introduction to Next Generation Sequencing
• Important things to consider when designing your Whole Genome Sequencing experiment
• Understanding the WGS-Seq workflow, analysis, and interpretation
• Other applications: Plasmid Sequencing & more
Duration: 30 minutes + Q&A
➜ Use promocode: WGS-Sept-2019 to receive 30% OFF any Whole Genome Sequencing, Plasmid Sequencing, or Mitochondrial DNA Sequencing Analysis service with us. Learn more about abm's NGS services at www.abmgood.co....
Register for the webinar to receive the presentation slides and other resources:
➜ info.abmgood.c...
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Пікірлер: 35

@abmgood 5 жыл бұрын

Useful timestamps: 0:00 Introduction 2:28 A Brief History of Genetics 4:34 Sanger Sequencing vs. Illumina Sequencing 8:40 Intro to Next Generation Sequencing 15:04 Important Considerations for Whole Genome Sequencing 17:04 Understanding the Workflow 27:00 Other Applications: Plasmid Verification, mtDNA-Seq 28:35 From the Human Genome Project to Today 30:14 Additional Resources and Conclusion

@AqleemAbbas 2 жыл бұрын

Whole genome means whole DNA or a gene of a DNA , part of gene is amplicon????

@CriticalTechReviews 3 жыл бұрын

Very helpful for a novice like me. I love your videos explaining the science so I know what I need, and your comprehensive services. I hope to get my project off the ground with your help soon.

@abmgood 3 жыл бұрын

Thanks so much for watching! ;) Glad you found the video helpful!

@ahmedg.hussain9699 4 жыл бұрын

This is an extraordinary and helpful webinar! It is by far the best I've seen on NGS and WGS! And I like the way the two presenters switch with their presentations! Well done to the team! The next content I would love to see (I hope I'm speaking for many viewers) is some insight into the analysis of the sequence data. Thank you!

@abmgood 4 жыл бұрын

Hi Ahmed, thank you for watching our webinar and leaving such a nice comment! Please let us know if you have any questions about the material and we will try our best to assist you!

@AmjadAli-zz1re Жыл бұрын

Welldone very helpful webinar regarding WGS, please arrange webinar on Multi locus sequence typing

@dnaseeker4873 2 жыл бұрын

Very helpful video, thank you. You talked about mitochondrial DNA at the end of the video. But is the mtDNA sequenced along with the nuclear DNA during whole genome sequencing or do you have to make another run ?

@spi3402 2 жыл бұрын

Very clear!!!!!!!!!!!!!

@abmgood 2 жыл бұрын

Thanks for watching!

@AmjadAli-zz1re Жыл бұрын

I just subscribed

@carlettagoodrich-mann1377 4 жыл бұрын

Lifestyle inherited structures can be modified. GENE DNA mutations can define systems functionality . SEQUENCING gene nucleotide Advantage’s could be the biological answers to creating a new recombinant for Corona . DNA platforms unveil the WHOLE genome that needs to be read. THANKS for the CME review

@bohe4581 4 жыл бұрын

Can you add subtitles to the video？This will make it clearer and easier to watch.

@abmgood 4 жыл бұрын

Hi Bo, if you click the "CC" button on the bottom right of the video player, there is an option to turn on subtitles for the video.

@jeanettewong7285 4 жыл бұрын

What strand does the fluorescent synthesis strand complement to? The reverse strand??? Once the fluorescent base is read do we have to infer the complement nucleotide to get the original template sequence?

@abmgood 4 жыл бұрын

This depends on which library prep kit is being used. For example, for Illumina's TruSeq mRNA Stranded kit, Read 1 corresponds to the reverse or antisense strand, while Read 2 corresponds to the forward or sense strand. In contrast, a library prepared with Illumina's Nextera Technology won't be stranded or directional. Other commercial kits may vary and it is best to check with the kit supplier for more information on their particular kit.

@esahkiddo 3 жыл бұрын

any video on new era sequencing ?

@aniellanazir1309 3 жыл бұрын

Hii like if we want to sequence whole genome of human like 50, having covid 19 symptoms half of them and half of them are asymtomatic. Which seq technique is good for them

@abmgood 3 жыл бұрын

Hello Aniella, This depends on the goal of your study. For example, Whole Genome Sequencing looks at the entire DNA genome, while Whole Exome Sequencing focuses on sequencing the exons only (i.e. protein coding regions). In contrast, RNA sequencing looks at RNA transcribed from DNA, some of which, but not all, derives from the exonic regions. For more information on the different sequencing techniques and its applications, please visit our Knowledge Base at: info.abmgood.com/next-generation-sequencing-ngs-experimental-design

@michaelqi5202 4 жыл бұрын

But what define the "sequence" ? Is it in 3D, 2D or time space? in other words, if one read AGT, what made that special order A-G-T? Why cannot it be read out as T-A-G ?

@rusticrick999 3 жыл бұрын

Because that is the order that the DNA polymerase or RNA polymerase reads the sequence, also known as the "sense" sequence. You don't read a book backwards, you start from page 1 and read to the last page.

@abmgood 3 жыл бұрын

Hello Michael, To determine the sequence, all four types of nucleotides are added during sequencing. After nucleotide incorporation, the remaining non-incorporated nucleotides are washed away. Next, a camera takes images of the fluorescently labeled nucleotides (i.e. fluorescent signal is read at each DNA cluster and recorded). The fluorescent molecule, along with the terminal 3' blocker, is then chemically removed from the DNA and washed away, allowing for the next cycle to begin. This process is repeated until the sequencing reaction is complete and allows for only a single nucleotide to be captured per cycle.

@nnnnmnn 3 жыл бұрын

TB whole genome sequencing

@jakubzahumensky8740 4 жыл бұрын

What is the point of the DNA forming bridges like this? And how are the bridges then disrupted for the chip to look as it does in fig 5?

@abmgood 4 жыл бұрын

19:30 - The goal of library prep is to create clusters of DNA instead of free floating DNA fragments, and Bridge PCR allows for cluster formation to occur. During library prep, two types of adapters are added to the DNA fragment, one adapter on each side of the fragment. Two types of oligos are also fixed on the flow cell (one forward and one reverse), with each oligo on the flow cell being complementary to each adapter. During amplification, the ssDNA fragments will bend or bridge over to reach nearby matching oligos on the flow cell, allowing for the amplified DNA to be in clusters. With normal PCR, the oligos are free floating in solution in the tube and do not allow for clusters to form. After amplification, the bridges are in the form of dsDNA. A denaturation step then occurs by increasing the temperature and dsDNA becomes ssDNA. The denaturation step leaves single stranded templates that are anchored to the substrate, allowing for the next round of amplification to occur, and eventually resulting in the flow cell looking like step 5.

@jakubzahumensky8740 4 жыл бұрын

@@abmgood Thank you.

@thaileonglai7812 Жыл бұрын

How does RNA contamination degrade our DNA samples?

@Raul28153 2 жыл бұрын

I had to listen to it over and over again the figure out that she was saying "throughput" around 5:00 Maybe clean up the narrative on these videos, people shouldn't have to struggle to understand.

@ekapurwanti2387 3 жыл бұрын

Assalamualaikum mohon ijin kami Jalasenastri Ny.eka Agus Riyanto mohon ijin bergabung'🙏

@chakri620 5 жыл бұрын

Chloroplast DNA

@abmgood 4 жыл бұрын

Hi there! Were you interested in chloroplast genome sequencing? If so, please contact our NGS Specialists at ngs@abmgood.com and they will be happy to assist you with your research.

@advancedcentercapacitybuil2183 4 жыл бұрын

the voice of the speaker (in the start) , her tone of voice and her pronunciation is really very annoying. addition of subtitles would be very helpful.

@abmgood 4 жыл бұрын

We'll take your feedback into account when we are working on our future videos! Meanwhile, you can try turning on the English (auto-generated) captions since we found them to be fairly accurate.

@sahrsuluku4585 4 жыл бұрын

Your comment is witless, everything about the first speaker was excellent.

@rusticrick999 3 жыл бұрын

Wow, how racist, grow up.