海洋学报(中文版)
海洋學報(中文版)
해양학보(중문판)
ACTA OCEANOLOGICA SINICA
2013年
4期
162-167
,共6页
李喜莲%张艳艳%辛静静%钱昭英%刘小林%相建海
李喜蓮%張豔豔%辛靜靜%錢昭英%劉小林%相建海
리희련%장염염%신정정%전소영%류소림%상건해
凡纳滨对虾%P23基因%抑制消减%生物信息学
凡納濱對蝦%P23基因%抑製消減%生物信息學
범납빈대하%P23기인%억제소감%생물신식학
Litopenaeus vannamei%P23 gene%bioinformatic%SSH
克隆凡纳滨对虾极端体重个体的组织差异表达基因 P23基因并进行生物信息学分析,为进一步研究该基因的功能以及凡纳滨对虾的分子选育等研究提供信息。以凡纳滨对虾雌虾极端体重个体腹部肌肉为实验材料,利用抑制消减杂交(SSH)技术构建极大体重雌性个体和极小体重雌性个体腹部肌肉组织正反向消减cDNA文库:正库(以极大体重个体为试验组,以极小体重个体为驱动组,L-S)和反库(以极小体重个体为试验组,以极大体重个体为驱动组,S-L)消减cDNA文库,并采用实时定量技术分析P23基因的组织表达规律,利用生物信息学对其功能和结构进行预测。以β-actin为看家基因检测两个文库的消减效率分别为210和25,实时定量技术分析结果表明 P23基因在体重的调节中起上调作用。P23基因编码区序列全长495bp ,编码165个氨基酸,GenBank登录号:JF806619。生物信息学分析发现P23蛋白部分序列含有强疏水性,无跨膜螺旋结构,两种信号肽预测都显示 P23含有信号肽。
剋隆凡納濱對蝦極耑體重箇體的組織差異錶達基因 P23基因併進行生物信息學分析,為進一步研究該基因的功能以及凡納濱對蝦的分子選育等研究提供信息。以凡納濱對蝦雌蝦極耑體重箇體腹部肌肉為實驗材料,利用抑製消減雜交(SSH)技術構建極大體重雌性箇體和極小體重雌性箇體腹部肌肉組織正反嚮消減cDNA文庫:正庫(以極大體重箇體為試驗組,以極小體重箇體為驅動組,L-S)和反庫(以極小體重箇體為試驗組,以極大體重箇體為驅動組,S-L)消減cDNA文庫,併採用實時定量技術分析P23基因的組織錶達規律,利用生物信息學對其功能和結構進行預測。以β-actin為看傢基因檢測兩箇文庫的消減效率分彆為210和25,實時定量技術分析結果錶明 P23基因在體重的調節中起上調作用。P23基因編碼區序列全長495bp ,編碼165箇氨基痠,GenBank登錄號:JF806619。生物信息學分析髮現P23蛋白部分序列含有彊疏水性,無跨膜螺鏇結構,兩種信號肽預測都顯示 P23含有信號肽。
극륭범납빈대하겁단체중개체적조직차이표체기인 P23기인병진행생물신식학분석,위진일보연구해기인적공능이급범납빈대하적분자선육등연구제공신식。이범납빈대하자하겁단체중개체복부기육위실험재료,이용억제소감잡교(SSH)기술구건겁대체중자성개체화겁소체중자성개체복부기육조직정반향소감cDNA문고:정고(이겁대체중개체위시험조,이겁소체중개체위구동조,L-S)화반고(이겁소체중개체위시험조,이겁대체중개체위구동조,S-L)소감cDNA문고,병채용실시정량기술분석P23기인적조직표체규률,이용생물신식학대기공능화결구진행예측。이β-actin위간가기인검측량개문고적소감효솔분별위210화25,실시정량기술분석결과표명 P23기인재체중적조절중기상조작용。P23기인편마구서렬전장495bp ,편마165개안기산,GenBank등록호:JF806619。생물신식학분석발현P23단백부분서렬함유강소수성,무과막라선결구,량충신호태예측도현시 P23함유신호태。
Screening ,cloning and bioinformatics analysis of P23 gene differently expressed in large female and small female of Litopenaeus vannamei.Suppression subtractive hybridization (SSH) approach was used to isolate differ-ently expressed genes in abdominal muscle samples of the female-shrimp between large female (LF;body weight>90 percentile of weight distribution curve) and small female (SF;body weight<10 percentile of weight distribution curve). Real-time reverse transcriptase-polymerase chain reaction (RT-PCR) was used to analysis the change of P23 mRNA level between large female and small female ,and biotechnology were employed to predict gene specific structure and potential motif domain.The subtraction efficiency was estimated by a housekeeping gene β-actin , and the results showed that β-actin was subtracted efficiently at 2 10 and 2 5 folds for SF and LF subtracted cDNA library respectively. RT-QPCR showed that the P23 has an effect to up-regulated expression in weight gain.Whole length of the P23 gene from Litopenaeus vannamei was 495bp (186 amino acid residues). The sequence has been accessed in GenBank (JF806619). Partial sequence of the P23 gene had strong hydrophobicity but with no transmembrane helices structure. The signal peptide prediction in P23 gene showed that there was a signal peptide with strong amino acid residues in the partial Sequence of the P 23 gene .
