Moderator: Charles Warden
Charles Warden ♦ 4.8k
- Reputation:
- 4,810
- Status:
- Trusted
- Location:
- Duarte, CA
- Website:
- https://sites.google.c...
- Twitter:
- @cwarden45
- Scholar ID:
- Google Scholar Page
- Last seen:
- 3 days, 9 hours ago
- Joined:
- 4 years, 1 month ago
- Email:
- c********@gmail.com
I am a Bioinformatics Specialist at City of Hope, where I work in the Integrative Genomics Core doing microarray and high-throughput sequencing analysis.
Posts by Charles Warden
<prev
• 607 results •
page 1 of 61 •
next >
0
votes
8
answers
38k
views
8
answers
... Yes - MATS will work without replicates.
If you do have replicates, [JunctionSeq][1] is also a relatively new option that I currently rank as my top choice for splicing analysis.
[1]: http://hartleys.github.io/JunctionSeq/ ...
written 19 days ago by
Charles Warden ♦ 4.8k
0
votes
2
answers
6.0k
views
2
answers
... Lowering the delta-beta cutoff will only help if the methylated thresholds are also changed. You could try setting both methyl.cutoff and unmethyl.cutoff equal to 0.3, or disable the use of methylated thresholds by setting unmethyl.cutoff=1 and methyl.cutoff=0.
Yes - in terms of posting etiquette, ...
written 5 weeks ago by
Charles Warden ♦ 4.8k
0
votes
1
answer
186
views
1
answers
... In most cases, it is difficult to confidently resolve classifications for 16S data at the species or sub-species level. So, if you were specifically interested in types of *Staphylococcus aureus*, it might be best to use a different marker (which you could define from comparing whole genome sequenc ...
written 7 weeks ago by
Charles Warden ♦ 4.8k
0
votes
2
answers
186
views
2
answers
... While I haven't directly used assemblage, I've done some testing with [MAKER][1], where I tended to get better results if I used protein / EST sequences (or an RNA-Seq *de novo* assembly) rather than starting with *de novo* gene predictions. Since it looks like assemblage is a modification of the M ...
written 10 weeks ago by
Charles Warden ♦ 4.8k
1
vote
1
answer
137
views
1
answers
... The R code that you are supposed to run is within the Word / PDF files, which call the other files under "R Tutorials"
At the beginning of the extracted R code, you'll need to define `dat0` as the beta matrix (such as `dat0 = read.table("probe_beta.txt",head=T, sep="\t")`)
Also, at least with the ...
written 10 weeks ago by
Charles Warden ♦ 4.8k
0
votes
2
answers
242
views
2
answers
Comment:
C: differential exon usage
... [DEXSeq][1] uses a specialized scripts (**dexseq_prepare_annotation.py** and **dexseq_count.py**) to run HTSeq for exon counts. The manual mentions that you can use other read counting programs, but I would typically use those specifically designed for DEXSeq (using a GTF annotation file).
Juncti ...
written 11 weeks ago by
Charles Warden ♦ 4.8k
1
vote
2
answers
242
views
2
answers
Answer:
A: differential exon usage
... If you are looking at differential exon usage (for patient characteristics, tumor-normal, etc.), DEXSeq is a popular option.
I happen to like [JunctionSeq][1] (which is based upon DEXSeq), which also includes splice sites (known junctions, and novel junctions between known exons) and an overall p-v ...
written 11 weeks ago by
Charles Warden ♦ 4.8k
0
votes
1
answer
132
views
1
answers
... Depends upon the library size - I believe the default setting is 3 cycles, and using 5 or 10 cycles is a little better if defining CCS reads. However, I typically don't see CCS reads greater than a few kb in length.
For genome assemblies, especially if you have 10+ kb segments of repetitive elemen ...
written 11 weeks ago by
Charles Warden ♦ 4.8k
2
votes
1
answer
183
views
1
answers
... The probe name indicates the methylation context, which can be either CpG or CpH (or a SNP probe with an rsID).
For example, ch.9.7776528F has hg19 coordinate chr9:7786528. The probe is for a CpH on the forward strand, so that position is a "C" and the next nucleotide is an "A" (H=A, C, or T).
In ...
written 4 months ago by
Charles Warden ♦ 4.8k
0
votes
1
answer
210
views
1
answers
... I would say it is OK to use CCS reads, where it might be a good idea to impose 5x or 10x cutoffs (the default is 3x).
I'm not as certain about error-corrected subreads if the library size is too large to define CCS reads. I guess it should be OK, but I can't really provide you with evidence from 1 ...
written 4 months ago by
Charles Warden ♦ 4.8k
Latest awards to Charles Warden
Teacher
6 days ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Teacher
5 weeks ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Good Answer
5 weeks ago,
created an answer that was upvoted at least 5 times.
For A: Your Favorite Bioinformatics Blog(S) (2013 Edition)
Appreciated
5 weeks ago,
created a post with more than 5 votes.
For A: A Practical (And Opinionated) Guide To Analyzing Human Methylation 450K Data
Great Question
9 weeks ago,
created a question with more than 5,000 views.
For How To Provide Reference Sequence Dictionary To Reordersam?
Teacher
10 weeks ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Popular Question
3 months ago,
created a question with more than 1,000 views.
For Memory Allocation for VarScan
Teacher
3 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Appreciated
4 months ago,
created a post with more than 5 votes.
For A: A Practical (And Opinionated) Guide To Analyzing Human Methylation 450K Data
Scholar
4 months ago,
created an answer that has been accepted.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Good Answer
4 months ago,
created an answer that was upvoted at least 5 times.
For A: Your Favorite Bioinformatics Blog(S) (2013 Edition)
Teacher
4 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Appreciated
4 months ago,
created a post with more than 5 votes.
For A: A Practical (And Opinionated) Guide To Analyzing Human Methylation 450K Data
Teacher
5 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Teacher
5 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Scholar
5 months ago,
created an answer that has been accepted.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Teacher
6 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Student
6 months ago,
asked a question with at least 3 up-votes.
For Gatk Error: Samfilereader Appears To Be Using The Wrong Encoding For Quality Scores
Teacher
7 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Popular Question
7 months ago,
created a question with more than 1,000 views.
For Solution: Gatk Doesn't Recognize Karyotypic Ordering
Appreciated
10 months ago,
created a post with more than 5 votes.
For A: A Practical (And Opinionated) Guide To Analyzing Human Methylation 450K Data
Scholar
10 months ago,
created an answer that has been accepted.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Teacher
11 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Teacher
11 months ago,
created an answer with at least 3 up-votes.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Scholar
12 months ago,
created an answer that has been accepted.
For A: Is it good idea to use two different quatification methods from TCGA at same tim
Use of this site constitutes acceptance of our User
Agreement
and Privacy
Policy.
Powered by Biostar
version 2.3.0
Traffic: 1120 users visited in the last hour