Construction of a muscle cDNA library of Chinese shrimp <Emphasis Type="Italic">Fenneropenaeus chinensis</Emphasis> and sequence analysis of the troponin I gene

A muscle cDNA library of Chinese shrimp (Fenneropenaeus chinensis) was constructed with the SMART™ cDNA Library Construction Kit. The titer of optimal primary library was 7.7×10⁵ pfu mL⁻¹ and that of the amplified library was 3.0×10⁹ pfu mL⁻¹. The percentages of the recombinant clones of primary and amplified libraries were over 98%. The insert sizes were longer than 400 bp with an average of 1000 bp. A positive clone containing a 794 bp insert was sequenced and identified encoding fast skeletal troponin I gene. This library provided a useful resource for the functional genomic research of F. chinensis.     

Construction of a Muscle cDNA Library of Chinese Shrimp Fenneropenaeus chinensis and Sequence Analysis of the Troponin Ⅰ Gene

A muscle cDNA library of Chinese shrimp (Fenneropenaeus chinensis) was constructed with the SMARTTM cDNA Li- brary Construction Kit. The titer of optimal primary library was 7.7×105 pfu mL-1 and that of the amplified library was 3.0×109 pfu mL-1. The percentages of the recombinant clones of primary and amplified libraries were over 98%. The insert sizes were longer than 400 bp with an average of 1000 bp. A positive clone containing a 794 bp insert was sequenced and identified encoding fast skeletal troponin Ⅰ gene. This library provided a useful resource for the functional genomic research ofE chinensis.     

南极冰藻 Chlamydomonas sp.ICE-L的 cDNA文库构建及品质检测

为构建南极冰藻Chlamydomonassp.ICE-L的cDNA文库,提取对数生长期南极冰藻ICE-L的总RNA,以此为模板,通过PowerScript逆转录酶逆转录合成第一链cDNA;再以第一链cDNA产物为模板,用LD-PCR合成第二链cDNA。该cDNA产物经分级分离转入大肠杆菌中,即获得南极冰藻ICE-L的cDNA原始文库,其滴度为1.6×106cfu/mL。扩增后的cDNA文库的滴度为1.0×1010cfu/mL。用PCR方法测得文库的重组率大于97%,插入cDNA的长度为0.5~1.8 kb,0.9 kb以上插入片段占50%以上。取适量扩增文库稀释并铺平板,挑取72个独立菌落,对其中22个独立菌落所插入的cDNA进行测序,克隆到了一个具有5′和3′非编码区的40S ribosomalprotein S5全长基因序列,GenBank收录号为AM167929。     

曼氏无针乌贼肌肉cDNA文库的构建和表达序列标签分析

以曼氏无针乌贼（Sepiellamaindroni）肌肉组织为研究材料,利用Clontech公司的cDNA文库构建试剂盒构建了曼氏无针乌贼肌肉cDNA文库．对文库质量的分析结果表明：cDNA文库的库容量约为1．2×10。克隆（cfu／dm^3）,重组率达96％,插入片段平均长度大于l000bp．挑取568个阳性克隆进行5’末端测序,其中475条ESTs长度大于100bp,初步拼接后得到200个单基因簇,包括41个重叠群和159个单拷贝EST,冗余度为57．89％．经检索,53条ESTs（占比为26．5％）在BLASTx上无明显的同源性（E值≥1．00×10^-10）,为新基因．147条ESTs（占比为73．5％）与已报道的基因有较高的同源性;其中与能量相关基因的ESTs丰度最高,占总数的23．0％．细胞信号传导、细胞骨架和蛋白质代谢的次之,比例分别为17．5％、12．5％、9．5％,其中包括热激蛋白70、转铁蛋白等．这些EST数据有助于进一步筛选和克隆曼氏无针乌贼和其他头足动物的肌肉特异性表达基因．