4.6 Article

De novo transcriptome sequencing and sequence analysis of the malaria vector Anopheles sinensis (Diptera: Culicidae)

期刊

PARASITES & VECTORS
卷 7, 期 -, 页码 -

出版社

BMC
DOI: 10.1186/1756-3305-7-314

关键词

Anopheles sinensis; Transcriptome; RNA-Seq; Codon usage bias; Simple sequence repeat; Malaria; Vector control

资金

  1. Par-Eu Scholars Program
  2. National Natural Science Foundation of China [31372265, 31200947]
  3. Coordinated Research Project of the International Atomic Energy Agency [18268/R0]
  4. National Institute of Health [R01 AI095184]
  5. Key Scientific and Technological Project of Chongqing [CSTC2012GG-YYJSB80002)]
  6. Natural Science Foundation Project of Chongqing [CSTC2013JCYJA00013]
  7. Science and Technology Project of Chongqing Municipal Education Commission [KJ130629]

向作者/读者索取更多资源

Background: Anopheles sinensis is the major malaria vector in China and Southeast Asia. Vector control is one of the most effective measures to prevent malaria transmission. However, there is little transcriptome information available for the malaria vector. To better understand the biological basis of malaria transmission and to develop novel and effective means of vector control, there is a need to build a transcriptome dataset for functional genomics analysis by large-scale RNA sequencing (RNA-seq). Methods: To provide a more comprehensive and complete transcriptome of An. sinensis, eggs, larvae, pupae, male adults and female adults RNA were pooled together for cDNA preparation, sequenced using the Illumina paired-end sequencing technology and assembled into unigenes. These unigenes were then analyzed in their genome mapping, functional annotation, homology, codon usage bias and simple sequence repeats (SSRs). Results: Approximately 51.6 million clean reads were obtained, trimmed, and assembled into 38,504 unigenes with an average length of 571 bp, an N50 of 711 bp, and an average GC content 51.26%. Among them, 98.4% of unigenes could be mapped onto the reference genome, and 69% of unigenes could be annotated with known biological functions. Homology analysis identified certain numbers of An. sinensis unigenes that showed homology or being putative 1: 1 orthologues with genomes of other Dipteran species. Codon usage bias was analyzed and 1,904 SSRs were detected, which will provide effective molecular markers for the population genetics of this species. Conclusions: Our data and analysis provide the most comprehensive transcriptomic resource and characteristics currently available for An. sinensis, and will facilitate genetic, genomic studies, and further vector control of An. sinensis.

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