What is sequencing depth? | Bioinformatics 101

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Bioinformagician

Bioinformagician

Күн бұрын

In this video I explain a term frequently used with sequencing i.e. depth associated with coverage (or depth of coverage, sequencing depth or read depth). In addition to discussing what these terms mean, I talk about what is the recommended coverage for different NGS data, how to visualize coverage and how to calculate coverage and coverage metrics from BAM files using samtools.
I hope you find this video helpful! Leave your thoughts in the comment section below!
Chapters:
0:00 Intro
0:32 What is coverage?
1:23 Depth of coverage (or sequencing depth)
1:49 Breadth of coverage
2:32 How to calculate coverage? (Lander/Waterman equation)
4:15 Recommended sequence coverage for NGS data
5:42 Visualizing coverage
6:17 Calculate coverage and coverage metrics
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#bioinformagician #bioinformatics #sequencing #coverage #samtools #depthofsequencing #samflag #sam #bam #alignment #phred #fasta #fastq #singlecell #10X #ensembl #biomart #annotationdbi #annotables #affymetrix #microarray #affy #ncbi #genomics #beginners #tutorial #howto #omics #research #biology #GEO #rnaseq #ngs

Пікірлер: 29
@crazychill6263
@crazychill6263 10 ай бұрын
I just wish I had someone like you to ask all my questions I´m completely lost in bioinformatics and it´s sooo hard to find someone to explain it to you in plain English or even find basic information 😐
@shobhitashah1929
@shobhitashah1929 Жыл бұрын
So far the best channel for genomics beginners!
@aamirmalik7740
@aamirmalik7740 2 жыл бұрын
Fantastic explanation of the concept -- please also continue with the lecture series you started on RNA Seq pipeline from scratch previously. Many Thanks
@user-lx3qr6zl7l
@user-lx3qr6zl7l 8 ай бұрын
your videos are extremely helpful! thank you so much ! i will follow your channels and watch every of your videos, please continue your update!
@tushardhyani3931
@tushardhyani3931 2 жыл бұрын
Thank you for this video !!
@sonalvishwakarma30
@sonalvishwakarma30 Жыл бұрын
Thanks! Please make more tutorials✨
@animatedbiologywitharpan
@animatedbiologywitharpan 2 жыл бұрын
Great explanation
@saurabhthakar
@saurabhthakar Жыл бұрын
Now I am assured that I am watching high-quality content because you are here.
@slendrmusic
@slendrmusic 8 ай бұрын
best bioinformatic channel
@mongekantorovich3555
@mongekantorovich3555 Жыл бұрын
Thank you!
@zlj8435
@zlj8435 2 жыл бұрын
Thanks a lot!
@nasreenbano523
@nasreenbano523 Жыл бұрын
Too good explanation. What will be the best recommended coverage for hi-C sequencing??
@hubijohn7451
@hubijohn7451 4 ай бұрын
awesome!
@sanjaisrao484
@sanjaisrao484 Жыл бұрын
Thanks
@Harshraj19988
@Harshraj19988 Жыл бұрын
I am trying to calculate the sequencing depth and coverage of WGBS data. I have bam files. So for samtools, input file is bam file or sorted bam file?
@shrijasrao9464
@shrijasrao9464 Жыл бұрын
what will the sequencing depth for wheat GBS ?
@emanuelavilla4733
@emanuelavilla4733 2 жыл бұрын
Great video! They are very useful, even to refresh the topic! I have a question, which may be a stupid one, but how do we decide the sequencing depth for single-cell RNA and ATAC? There are any recommendations?
@Bioinformagician
@Bioinformagician 2 жыл бұрын
Excellent question! I do not think there is a straightforward formula or criteria to answer that question. I think there are a lot of factors involved like (and not limited to) heterogeneity of population cells (whether one is trying to identify rare cells populations), whether certain genes are expressed at high level in the condition or population you are investigating (if one is trying to investigate if a certain gene is expressed in certain cell population), sample type library, platform and cost. Of course there are recommended sequencing depths for single-cell RNA and ATAC libraries, but ultimately depth has to be adjusted based on the application and budgeting constraints. I am linking some articles which may be of interest - genomemedicine.biomedcentral.com/articles/10.1186/s13073-017-0467-4 www.nature.com/articles/nbt.3039#:~:text=Large%20sample%20sizes%20impose%20a,reads%20per%20cell%20may%20suffice. www.10xgenomics.com/support/single-cell-multiome-atac-plus-gene-expression/documentation/steps/sequencing/sequencing-requirements-for-single-cell-multiome-atac-plus-gene-expression kb.10xgenomics.com/hc/en-us/articles/115002022743-What-is-the-recommended-sequencing-depth-for-Single-Cell-3-and-5-Gene-Expression-libraries-
@anamikapandey4769
@anamikapandey4769 Жыл бұрын
great lecture😍, please make a video on ChiP SEQ data analysis.....it will be more helpful for us
@Bioinformagician
@Bioinformagician Жыл бұрын
That is definitely in the pipeline. Please stay tuned :)
@anamikapandey4769
@anamikapandey4769 Жыл бұрын
@@Bioinformagician thank you💜
@davidtupatron
@davidtupatron 2 ай бұрын
Great video! You literally clarify everything! I have a question, what woukd be the recommended depth for assessment of SNPs in a amplicon sequence? 🤔 and also, does the error rate play a role in getting the depth? I hope you could answer my question! Thank youuuu
@javiersanjuan296
@javiersanjuan296 8 ай бұрын
How can I calculate coverage for amplicon sequencing if I have multiple amplicons of different sizes pooled together? Should I use an average size for all the amplicons?
@ch00p
@ch00p Жыл бұрын
At 4:11 why is the coverage for the single bp region 5X? LG/N = 8(5)/1=40X. Is this just an exception for single nucleotide regions?
@Bioinformagician
@Bioinformagician Жыл бұрын
It's an exception for single nucleotide regions.
@AyrodsGamgam
@AyrodsGamgam Жыл бұрын
it's 1(5)/1=5X, because it's only one nt
@Fabiano1012
@Fabiano1012 2 жыл бұрын
👏👏👏👏
@juanete69
@juanete69 28 күн бұрын
Why is it important the direction of the read?
@himanshusaxena387
@himanshusaxena387 Жыл бұрын
It's a fine video, but it sounds more bookish. Should try to express more simply (language particlarly) and graphically.
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