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Identification of testis-relevant genes using in silico analysis from testis ESTs and cDNA microarray in the black tiger shrimp ( Penaeus monodon)

机译:利用计算机分析从黑虎虾(斑节对虾)睾丸EST和cDNA芯片中进行的睾丸相关基因鉴定

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Poor reproductive maturation of the black tiger shrimp (Penaeus monodon) in captivity is one of the serious threats to sustainability of the shrimp farming industry. Understanding molecular mechanisms governing reproductive maturation processes requires the fundamental knowledge of integrated expression profiles in gonads of this economically important species. In P. monodon, a non-model species for which the genome sequence is not available, expressed sequence tag (EST) and cDNA microarray analyses can help reveal important transcripts relevant to reproduction and facilitate functional characterization of transcripts with important roles in male reproductive development and maturation. In this study, a conventional testis EST library was exploited to reveal novel transcripts. A total of 4,803 ESTs were unidirectionally sequenced and analyzed in silico using a customizable data analysis package, ESTplus. After sequence assembly, 2,702 unique sequences comprised of 424 contigs and 2,278 singletons were identified; of these, 1,133 sequences are homologous to genes with known functions. The sequences were further characterized according to gene ontology categories (41% biological process, 24% molecular function, 35% cellular component). Through comparison with EST libraries of other tissues of P. monodon, 1,579 transcripts found only in the testis cDNA library were identified. A total of 621 ESTs have not been identified in penaeid shrimp. Furthermore, cDNA microarray analysis revealed several ESTs homologous to testis-relevant genes were more preferentially expressed in testis than in ovary. Representatives of these transcripts, homologs of saposin (PmSap) and Dmc1 (PmDmc1), were further characterized by RACE-PCR. The more abundant expression levels in testis than ovary of PmSap and PmDmc1 were verified by quantitative real-time PCR in juveniles and wild broodstock of P. monodon. Without a genome sequence, a combination of EST analysis and high-throughput cDNA microarray technology can be a useful integrated tool as an initial step towards the identification of transcripts with important biological functions. Identification and expression analysis of saposin and Dmc1 homologs demonstrate the power of these methods for characterizing functionally important genes in P. monodon.
机译:被圈养的黑虎虾(斑节对虾)繁殖不佳是对虾养殖业可持续性的严重威胁之一。要了解控制生殖成熟过程的分子机制,需要具备该经济上重要物种的性腺中完整表达谱的基础知识。在斑节对虾(P. monodon)中,无模型物种的基因组序列不可用,表达序列标签(EST)和cDNA微阵列分析可帮助揭示与生殖有关的重要转录本,并促进在雄性生殖发育中具有重要作用的转录本的功能表征和成熟。在这项研究中,传统的睾丸EST文库被用来揭示新的成绩单。使用可定制的数据分析包ESTplus,对总共4,803个EST进行了单向测序并进行了计算机分析。序列组装后,鉴定了由424个重叠群和2278个单例组成的2702个独特序列。其中1,133个序列与具有已知功能的基因同源。根据基因本体论类别(41%的生物过程,24%的分子功能,35%的细胞成分)进一步表征序列。通过与斑节对虾其他组织的EST文库进行比较,鉴定出仅在睾丸cDNA文库中发现的1579个转录物。尚未在对虾中鉴定出总共621个EST。此外,cDNA微阵列分析显示,与睾丸相关基因同源的几个EST在睾丸中比在卵巢中更优先表达。这些转录物的代表,saposin(PmSap)和Dmc1(PmDmc1)的同源物,通过RACE-PCR进一步表征。通过定量实时荧光定量PCR证实了斑节对虾幼体和野生亲体中睾丸中的表达水平高于卵巢中PmSap和PmDmc1的表达水平。如果没有基因组序列,则EST分析和高通量cDNA微阵列技术的结合可能是有用的集成工具,是鉴定具有重要生物学功能的转录本的第一步。 saposin和Dmc1同源物的鉴定和表达分析证明了这些方法表征斑节对虾功能上重要基因的能力。

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