棉铃虫普通气味受体基因HarmOR9和HarmOR29的克隆和组织表达分析

【目的】对棉铃虫Helicoverpa armigera 2个普通气味受体基因的cDNA全长进行分析,明确这两个普通气味受体基因在不同组织中的表达分布,为进一步的功能研究奠定基础。【方法】利用PCR结合RACE技术克隆棉铃虫两条普通气味受体基因的cDNA全长;利用不同的生物信息学软件对序列进行结构预测、序列比对和进化树分析;利用半定量RT-PCR检测其在棉铃虫成虫不同组织中的表达。【结果】获得两条棉铃虫气味受体基因的全长序列,并命名为HarmOR9和HarmOR29（GenBank登录号分别为KJ188252和KJ188253）。序列分析显示,HarmOR9全长1 206 bp,编码401个氨基酸;HarmOR29全长1 188 bp,编码395个氨基酸。选择已报道的鳞翅目昆虫烟青虫Heliothis assulta、家蚕Bombyx mori、烟芽夜蛾Heliothis virescens和棉铃虫的气味受体与本实验克隆得到的两个气味受体基因的编码产物进行序列比对和进化树分析,结果显示这两个气味受体与性信息素受体区别明显,并与其他普通气味受体聚类在一起。半定量RT-PCR的结果显示HarmOR9与HarmOR29都主要在触角中高表达且无雌雄间差异,HarmOR29在其他组织中均不表达;而HarmOR9在雄虫下唇须中有微量表达,在其他组织中均不表达。【结论】本研究从棉铃虫中克隆得到2个气味受体基因HarmOR9和HarmOR29的cDNA全长,其编码产物具有气味受体的典型特征并且属于普通气味受体。明确了这两个气味受体基因都在棉铃虫成虫的触角中高表达,且无雌雄差异,推测其可能参与了棉铃虫普通气味的识别过程。     

白纹伊蚊细胞色素P450 CYP6家族基因多样性的研究(英文)

根据已获得的白纹伊蚊CYP6家族某成员cDNA序列片段AEDR ,设计基因特异性引物 ,以白纹伊蚊总RNA为模板 ,进行cDNA末端快速扩增 ,扩增产物经T -A克隆、测序。结果显示 :通过 5’ RACE获得 1个非全长cDNA序列 (GZS331 ) ,其与CYP6N1、CYP6N2的同源性分别为 59 8%和 59 1 % ,与CYP6N3v1 -v3同源性最高 ,达 83 9% - 84 3% ;通过 3’ RACE获得 6个非全长cDNA序列 ,其中来自抗性株的GZG0 33序列与CYP6N3v1 -v3的同源性达 98 2 % - 99 1 % ,而其余 3’ RACE克隆与CYP6N3v1 -v3的同源性则达 84 3% - 85 6%。上述所有非全长cDNA序列均与哺乳动物CYP3A1以及夜蛾CYP9A1有较高的同源性 ,分别为 2 3% - 36 1 %和 2 7 6% - 34 1 %。用PC/GENE软件所绘制的系统树显示出与同源性分析相一致的结果。所得非全长cDNA序列上报国际P450命名委员会进行统一的命名 ,并对蚊虫中细胞色素P450基因多样性及其形成原因进行了分析     

Cloning of GT box-binding proteins: a novel Sp1 multigene family regulating T-cell receptor gene expression.

Analysis of a T-cell antigen receptor (TCR) alpha promoter from a variable gene segment (V) revealed a critical GT box element which is also found in upstream regions of several V alpha genes, TCR enhancer, and regulatory elements of other genes. This element is necessary for TCR gene expression and binds several proteins. These GT box-binding proteins were identified as members of a novel Sp1 multigene family. Two of them, which we term Sp2 and Sp3, were cloned. Sp2 and Sp3 contain zinc fingers and transactivation domains similar to those of Sp1. Like Sp1, Sp2 and Sp3 are expressed ubiquitously, and their in vitro-translated products bind to the GT box in TCR V alpha promoters. Sp3, in particular, also binds to the Sp1 consensus sequence GC box and has binding activity similar to that of Sp1. As the GT box has also previously been shown to play a role in gene regulation of other genes, these newly isolated Sp2 and Sp3 proteins might regulate expression not only of the TCR gene but of other genes as well.     

Drosophila melanogaster genes for U1 snRNA variants and their expression during development.

We have cloned and characterized a complete set of seven U1-related sequences from Drosophila melanogaster. These sequences are located at the three cytogenetic loci 21D, 82E, and 95C. Three of these sequences have been previously studied: one U1 gene at 21D which encodes the prototype U1 sequence (U1a), one U1 gene at 82E which encodes a U1 variant with a single nucleotide substitution (U1b), and a pseudogene at 82E. The four previously uncharacterized genes are another U1b gene at 82E, two additional U1a genes at 95C, and a U1 gene at 95C which encodes a new variant (U1c) with a distinct single nucleotide change relative to U1a. Three blocks of 5' flanking sequence similarity are common to all six full length genes. Using specific primer extension assays, we have observed that the U1b RNA is expressed in Drosophila Kc cells and is associated with snRNP proteins, suggesting that the U1b-containing snRNP particles are able to participate in the process of pre-mRNA splicing. We have also examined the expression throughout Drosophila development of the two U1 variants relative to the prototype sequence. The U1c variant is undetectable by our methods, while the U1b variant exhibits a primarily embryonic pattern reminiscent of the expression of certain U1 variants in sea urchin, Xenopus, and mouse.     

Arabidopsis thaliana vegetative storage protein (VSP) genes: gene organization and tissue-specific expression

We have previously identified two cDNAs encoding vegetative storage proteins (VSPs) in Arabidopsis thaliana. Unlike soybean in which VSPs accumulate at high levels in leaves, A. thaliana VSP mRNAs are abundant in flowers. To understand tissue-specific expression and possible roles of VSPs on reproductive organ development, genes corresponding to VSPs (Vsp1 and Vsp2) and their putative promoters were characterized in this study. Genomic sequence analysis revealed that Vsp1 and Vsp2 resemble each other except in their introns, and that these two genes were organized in a tandem array with an interval of 6 kb in a region. The expression patterns of Vsp1 and Vsp2 were examined using transgenic A. thaliana plants carrying a promoter from Vsp1 or Vsp2 fused to a bacterial -glucuronidase (GUS) reporter gene. The promoter from Vsp1 expressed its effect in gynoecia, especially in styles, the basal and distal ends of ovaries and in siliques, whereas the promoter from Vsp2 showed its activity in vegetative shoots, petioles, peduncles and receptacles of floral organs. These results suggest that expression of Vsp1 and Vsp2 may be developmentally regulated in A. thaliana. In the transgenic plants, the GUS activity was induced by wounding in an area around the mid-rib of leaves. Therefore, Vsp1 and Vsp2 promoters appear to have elements required for both tissue specificity and wounding.     

Divergence and differential expression of soybean actin genes

DNA sequence analysis as well as genomic blotting experiments using cloned soybean actin DNA sequences as probes show that large sequence heterogeneity exists among members of the soybean actin multigene family. This heterogeneity suggested that the members of this family might be diverged in function and/or regulation. Five of the six soybean actin gene family members examined are shown to be significantly more diverged from one another than members of other known actin gene families. This high level of divergence was utilized in the preparation of actin gene-specific probes in the analysis of the complexity and expression of these members of the soybean actin gene family. Hybridization studies indicate that the six soybean actin genes fall into three classes with a pair of genes in each class. These six genes account for all but two actin gene fragments detected in the soybean genome. We have compared the relative steady state mRNA levels of these classes of soybean actin genes in three organs of soybean. We find that actin genes SAc6 and SAc7 are most highly expressed accounting for 80% of all actin mRNA with respect to the six soybean actin genes examined. Actin genes SAc3 and SAc1 are expressed at intermediate and low levels respectively; and SAc2 and SAc4 are expressed at barely detectable levels. Four of the six soybean actin genes appear to be expressed at the same level in root, shoot and hypocotyl. SAc3 and SAc7 genes appear to be more highly expressed in shoot and 2,4-dichlorophenoxyacetic acid-induced hypocotyl than in root and hypocotyl.(ABSTRACT TRUNCATED AT 250 WORDS)