Feb

14

Life Technologies weighs in on Roche – Illumina Deal

Filed Under News 

Last week an article appeared in BioArray News as part of the coverage of the ongoing Roche/Illumina story – Illumina Array Customers ‘Apprehensive’ of Possible Roche Takeover, Fear Platform ‘Stagnation’

Yesterday, I received an email from Life Technologies (I guess I’m on their marketing list) that seemed unusual to me.  No message, just an image with a link to the article.

life technologies

This email was clearly intended to draw attention to the article and highlight the fears of current Illumina customers about the possible deal.  Were they trying to build opposition to the deal?  Do they feel the combined financial strength of Roche and the technical strength of Illumina would be a formidable competitor?  You decide…

Incoming search terms:

  • roche life technologies
  • life technologies roche
  • illumina vs life technologies
  • roche to buy life technologies
  • roche buy life technologies
  • roche life tech
  • roche and life technologies
  • life technologies vs illumina
  • life tech roche
  • life technologies takeover

Comments

Leave a Reply




  • Social Networking Pages

    Linkedin Group

  • Follow Me on Pinterest

  • RSS SEQanswers – RNA Sequencing

    • HT Seq Count stranded options May 24, 2013
      I am very new to bioinformatics, so I would be really grateful for some help! I have been using *HTSeq Count v0.5.3* and I am bit confused about... […]
      qwrissie
    • Tophat 2.0.8b installation error May 24, 2013
      I install tophat-2.0.8b to rerun the mapping. but when i make it, the error appears like this. make[1]: Entering directory... […]
      canhu
    • reason for low mapping rate?? May 23, 2013
      we did RNASeq using HiSeq 2000 100PE. When the data were back, I mapping them to the reference sequence, but got very low mapping rate (30-40%). I... […]
      miaom
    • cross-species data - questions about normalization May 23, 2013
      Hi, I have some data form various samples (cell types) in different species. I want to compare and analyze gene expression variability across the... […]
      trelek2
    • CuffDiff strange output May 23, 2013
      Hi, I hope that someone can be so gentle to help me. I'm analizing some data from RNA-Seq with TopHat and Cufflinks and I focus my attention on... […]
      Pruexel
    • cannot away with cuffdiff,incredible May 23, 2013
      Hi,all I have 4(A,B,C,D) sample in 4 times(increasing time),I got diff result in 3 different cuffdiff 1.cuffdiff 3(A,B,C) individual... […]
      upper

  • RSS Biostar – RNA-Seq

    • Why am I getting so many unmapped reads in STAR, classified as "too short"?
      I am currently using STAR to map several Hi-SEQ mRNA runs. I'm having trouble getting a decent amount of reads to map, but I don't really understand why. I'm hoping you can shed some light :) In the final log, only about 50% (or less) of the reads map to the reference. I'm using a GTF in addition to the genome. The unmapped bin that most […]
    • What are the best practices for SNP identification in RNA seq transcriptome data
      I have 20 RICE RNA seq tranascriptome data hiseq 2000 platform paired end reads. I aligned fasta reads with BWA and remove PCR duplicates with PICARD. Later I call SNP with samtools using various parameters. I would like to clarify what parameters should I used while alinging to reference rice genome for looking SNP location 100 bp upstream and 250 bp downst […]
    • How do TopHat options -g , --supress-hits, and Bowtie options interplay?
      Hi, I am currently using TopHat2 to map RNA-seq runs. I think there have been some changes pertaining the -g option. Does anyone know how it works now? I used to think that setting -g would look for n alignments for a given read, report them [if top-scoring] and discard those reads that had more than g [top scoring] alignments. Now, the description sounds mo […]
    • What happened to -k in TopHat for multiple-mapping reads?
      Selecting -g n in tophat does not discard reads mapping more than n, but instead only reports n alignments for those out all all their TOP scoring alignments. I think there used to be an option -k that would allow one to discard reads that topped x alignments -- whatever happened to that? I only see -g in the tophat 2 manual, no reporting options like before […]
    • Does tophat use the library-type information for mapping, or just for the XS flag?
      When I specify library-type to TopHat, i.e., first-strand, second-strand, unstranded, TopHat appends a value + or - to the XS:A flag, which is useful for subsequent analyses, such as annotation. However, does this information actually influence the "mappability" of reads, or is this unaffected? My thinking is that the information would be considere […]
    • Purpose of Y-shaped adapters in Illumina Sequencing?
      Hi all, Y adapters different sequences to be annealed to the 5' and 3' ends of each molecule in a library. The arms of the Y are unique, and the middle part, connected to the DNA fragment, is complementary. What are the advantages of this? My take of this over having fully-complementary adapters (ADAPTER1 - - - - - ADAPTER1) is that: -Upon primer a […]