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1.
从猪胚胎骨骼肌cDNA文库中筛选出一克隆子,通过测序及电子延伸获得包含全长CDS的猪VDAC1基因cDNA序列。比对发现此基因在核苷酸和氨基酸水平与人及小鼠都具有较高的同源性。应用辐射杂种板(RH)对此基因进行染色体的精确定位,定位结果显示VDAC1基因定位在猪2号染色体长臂。  相似文献   

2.
猪CACNA1S基因部分序列的克隆、测序及SNP检测   总被引:2,自引:0,他引:2  
CACNA1S是钙离子通道主效亚基α1亚单位的编码基因,该基因突变会导致人(Homo sapiens)低钾性周期性麻痹和恶性高温综合征.目前CACNAIS基因的研究主要集中在人和模式动物上,而在家畜中的研究少见报道.本研究以金华猪(115头)、皮特兰猪(30头)、金华猪与皮特兰猪杂交产生的金皮F2代杂种猪(126头)、大约克猪(23头)为研究对象,根据人CACNA1S基因序列设计引物,对猪基因组DNA进行PCR扩增、克隆测序,并与人相应序列作同源性比较,然后采用PCR-SSCP技术检测序列中可能存在的单核苷酸多态(single nucleotide polymorphism,SNP)位点,并对有合适内切酶存在的突变点应用PCR-RFLP技术进行验证.结果表明:(i)用6对引物对猪基因组DNA进行扩增,共克隆得到猪CACNAIS基因约5211bp的DNA序列,其中外显子区域,猪与人同源性为82.6%,序列已递交GeneBank收录(登录号DQ767693);(ii)在克隆得到的DNA序列中,共检测到57个单核苷酸突变点,其中外显子区域存在24个;(iii)突变位点的PCR-RFLP验证与PCR-SSCP检测结果一致,经与GenBank公布的猪CACNAIS基因EST小片段(Bx914582,Bx666997)比较,相应长度核酸序列内本实验检测到的11个SNP位点中,有8个位点的碱基突变与2个EST片段间存在的碱基差异相同.  相似文献   

3.
对丹参EST数据库进行BLAST同源性比对发现,登录号为CV165156的EST序列与硫氧还蛋白基因(Trx)有很高的同源性。进一步用PCR方法从丹参基因组水平上克隆到长1806bp的DNA序列(登录号为FJ217699),与cDNA序列比对发现,该基因(SmTrxh)含有2个内含子。生物信息学分析表明,SmTrxh所编码蛋白的分子质量为13.4kDa,理论等电点为5.53,无信号肽,属于定位于细胞质中的稳定类蛋白。该蛋白与其他7种植物中的Trx高度同源,同源性介于68%-74%之间。实时定量PCR检测的结果显示,SmTrxh在丹参中为组成型表达基因,在根、茎和叶中都有表达,主要在根部表达,茎中的表达量最低。  相似文献   

4.
利用抑制性消减杂交技术 (suppression subtractive hybridization , SSH) 成功地构建了双肌臀与非双肌臀大白猪肌肉组织差异表达的消减 cDNA 文库,获得有效克隆 686 个. 对整个文库测序分析,共获得 587 条有效序列. 利用 BLAST 在线软件与 GenBank、 GenBank EST 和 Tigr Porcine EST 等数据库进行同源序列比较,发现其中有 11 个未知新序列,可能代表“双肌臀”大白猪肌肉组织特异表达的新基因. 对文库中所包含的兰尼啶受体基因 (RYR1)、钙依赖性蛋白激酶 基因 (CAMK2)、人类胰岛素生长因子结合蛋白 -7 基因 (IGFBP7),以及 695号、 882号和480号3个新基因进行了实时荧光定量 PCR 检测,结果显示: RYR1、 CAMK2 及 IGFBP7 基因在双肌臀猪肌肉组织 RNA 池中的表达量,分别为对照的非双肌臀猪肌肉组织 RNA 池中表达量的 1.87、 1.90 和 1.85 倍; 695 号、 882 号和 480 号 3 个新的 ESTs 在双肌臀猪肌肉组织 RNA 池中的表达量为非双肌臀猪肌肉组织 RNA 池中表达量的 1.48、 1.44 和 1.78 倍. 这提示我们,上述基因的上调表达很可能与猪双肌臀性状的发生有密切的关系,可以作为研究该性状的候选基因.  相似文献   

5.
猪脂肪组织表达序列标签(ESTs)大规模测序及分析   总被引:1,自引:0,他引:1  
邓亚军  童维  陈雁炯  胡松年  李生斌 《遗传学报》2004,31(11):1211-1217
利用大规模DNA序列测定的方法,对猪脂肪组织进行了表达序列标签(Expressed Sequence Tag,EST)序列测定,获得高质量EST共7790个,并对此进行了初步分析。使用STACK-PACK软件进行聚类分析,得到4354个基因聚类,包括3609个单拷贝基因和745个多拷贝基因;将候选基因序列用BlastN与nr库进行比较(e=1e-10),从4354个候选基因中得到2712个已知基因,其中单基因为1987个,多拷贝基因为725(3694克隆)个;未知功能基因和新EST有2109个克隆。根据BlastN结果,利用基因组文库添加序号(GenBank Accession No.)为索引,构建了猪脂肪组织已知功能基因表达谱。从基因表达谱可以看出,在猪脂肪组织中参与代谢的基因所占比例最高,在某些方面也显示了脂肪组织旺盛的代谢活性。同时发现在猪脂肪组织中主组织相容性抗原(Major Histocompatibility Complex,MHC)或与MHC相关的基因表达丰度很高。其中单拷贝基因181个,多拷贝基因44个,共计257个克隆,占细胞机体防御(cell and organism defense)总数的44.9%。占总已知基因数的5.4%。提取出全部与MHC相关的EST序列(257个克隆),发现所有EST的部分序列(长约200个碱基),几乎分布在每一个已知猪BAC的所有编码序列上。据此推测,构成MHC的这些EST序列中,有一段长约200个碱基(200bp)的碱基序列高度保守,MHC基因中每一段编码序列都包含有这一段序列。这些MHC序列虽然在不同的BAC上其蛋白的域不同,但均为高度保守区域,并且都与免疫功能密切相关。猪脂肪中如此大量表达的MHC部分保守序列,由于与免疫功能高度相关,在MHC基因的传递过程中,可以反复复制,并能够稳定遗传。  相似文献   

6.
猪骨骼肌快肌肌钙蛋白C2基因的cDNA克隆与表达分析   总被引:3,自引:0,他引:3  
从人骨骼肌快肌肌钙蛋白C2(TNNC2)基因出发,在dbEST数据库中进行同源性搜索,找到一个有较高同源性且在猪背最长肌中表达EST(BM083186)。通过电子克隆和进一步RT-PCR实验验证,获得猪TNNC2基因全长cDNA序列,其全长843bp,开放阅读框为201~683bp,编码有160个氨基酸。同源性分析结果表明,与人、鼠的骨骼肌快肌肌钙蛋白C2基因cDNA编码区(CDS)同源性分别为93.6%、90.5%,蛋白序列同源性均为97.5%。多种组织的半定量RT-PCR研究表明,该基因在骨骼肌中表达,并且在杜洛克猪背最长肌中的表达比兰塘猪高。  相似文献   

7.
利用5'/3'RACE FCR技术,从桃(Prunus persica(L.)Batsch)果实中克隆了植物乙烯生物合成的关键酶-ACC合酶的全长cDNA pacs,对pacs基因进行全序列测定表明,该基因全长1848个碱基,编码区1449个碱基,5'端有177个碱基的非编码区序列,3'端有219个碱基的非编码区序列(不包括终止密码子TAA)。pacs基因编码区共编码483个氨基酸,蛋白质大小为54kd,等电点为6.43。pacs与番茄(S19677)、梅(AB031026)、番木瓜(U68216)、苹果(AB034993)等其他植物ACC合酶cDNA氨基酸序列同源性分别为65%、70%、90%,并存在与这些ACC合酶氨pacs12(af467782)在叶片和花中基因表达模式基本一致,伤处理和IAA均能诱导叶片pacs和pacs12基因的表达,但pacs在伤处理叶片的表达水平比pacs12高;pacs和pacs12基因在果实表达有所不同,pacs在绿熟和成熟果实中均有表达,而pacs12在绿熟果实中基本检测不同,在成熟果实中才有表达,两在果实中的表达水平比伤处理和IAA处理叶片和花中要低。  相似文献   

8.
目的:Aspergillus niger(CU-1)菌株α-葡萄糖苷酶基因(agdA)克隆并对其序列进行分析,构建该基因的真核表达载体。方法:设计合成的一对特异性引物,采用PCR以总DNA为模板,扩增得到DNA片段(D1);采用RT-PCR方法扩增得到DNA片段(D2)。将DNA片段D1和D2转入大肠杆菌中并进行了序列测定,序列进行BLAST比对分析。将α-葡萄糖苷酶基因的cDNA片段与表达载体pGAPZαA连接,构建重组表达载体。结果:基因agdA大小为3 127bp,含有3个外显子和4个内含子。该基因的cDNA序列大小为2 958bp,包含完整的编码框,编码985个氨基酸。agdA基因序列与已发表的α-葡萄糖苷基因序列同源性达99%,其中有6个位置的碱基发生了变化。已成功构建重组表达载体pGAPZαA-agdA。结论:Aspergillus niger(CU-1)菌株α-葡萄糖苷酶基因序列分析及重组表达载体pGAPZαA-agdA的构建为在毕赤酵母中表达Aspergillus niger(CU-1)菌株的α-葡萄糖苷酶奠定基础。  相似文献   

9.
Ⅱ型启动子转录的外源短链RNA可以竞争性抑制细胞内源mRNA的核质转运,因而可能会提高植物RNA 病毒载体表达的外源基因在植物中的积累. 为了验证这一假说,利用OE-PCR技术合成拟南芥U6-1核内小RNA序列,并构建其Ⅱ型启动子转录的植物表达载体. 以农杆菌渗滤技术,与烟草花叶病毒(Tobacco mosaic virus, TMV)表达载体共接种寄主植物本氏烟,通过对报告基因绿色荧光蛋白(green fluorescence protein, GFP)的荧光观察,并以Western印迹和ELISA测定GFP在烟草中的表达情况,分析共表达Ⅱ型启动子转录的U6 RNA对外源基因在植物中表达的作用效果. 结果表明,共接种Ⅱ型启动子转录的U6 RNA对TMV病毒表达载体表达外源基因的水平有明显的增效作用,推测RNA核质转运干扰是提高外源基因表达的可能机制.  相似文献   

10.
猪脂肪及肌肉组织中基因表达信息分析   总被引:1,自引:0,他引:1  
为探测猪脂肪及肌肉组织中基因表达概况,利用猪EST资源和人类基因序列开展计算机模拟研究,旨在为猪肉质改良的遗传基础分析提供候选信息。执行Blast比对程序以识别人类基因组基因与猪EST序列间的同源性并筛选出高度同源记录,同时编制4个Java程序进行序列检索收集、序列比对结果的过滤筛选以及分类处理。统计分析表明:至少有2002个基因在猪脂肪及肌肉组织中表达,其中1087个基因在脂肪组织表达,1205个基因在肌肉组织中表达,两组织共同表达的基因为290个;筛选出高同源基因,同时分类统计出了114个基础活性基因(脂肪和肌肉组织分别表达80和34个),并选取Top记录进行了描述分析和总结。  相似文献   

11.
Conserved segments have been identified by ZOO-FISH between pig chromosome 9 (SSC9) and human chromosomes 1, 7 and 11. To assist in the identification of positional candidate genes for QTL on SSC9, the comparative map was further developed. Primers were designed from porcine EST sequence homologous to genes in regions of human chromosomes 1, 7 and 11. Porcine ESTs were then physically assigned using the INRA somatic cell hybrid panel (INRASCHP) and the high-resolution radiation hybrid panel (IMpRH). Seventeen genes (PEPP3, RAB7L1, FNBP2, MAPKAPK2, GNAI1, ABCB1, STEAP, AKAP9, CYP51A1, SGCE, ROBO4, SIAT4C, GLUL, CACNA1E, PTGS2, C1orf16 and ETS1) were mapped to SSC9, while GUSB, CPSF4 and THG-1 were assigned to SSC3.  相似文献   

12.
We report the chromosomal assignment of 18 porcine genes to human homologues using the INRA-Minnesota swine radiation hybrid panel (IMpRH). These genes (CACNA1C, COL2A1, CPNE8, C3F, C12ORF4, DDX11, GDF11, HOXC8, KCNA1, MDS028, TMEM106C, NR4A1, PHB2, PRICKLE1, Q6ZUQ4, SCN8A, TUBA8 and USP18) are located on porcine chromosome 5 (SSC5) and represent positional and functional candidates for arthrogryposis multiplex congenita (AMC), which maps to SSC5. CPNE8, PRICKLE1, Q6ZUQ4 and TUBA8 were mapped to the interval for pig AMC between microsatellites SW152 and SW904. Three SNPs in TUBA8 co-segregated with the AMC phenotype in 230 pigs of our research population without recombination and could be used as a genetic marker test for AMC. In addition, we provide evidence that a small chromosomal region of HSA22q11.2 evolutionarily corresponds to SSC5q12-q22 (and contains the human homologues of porcine SW152, Q6ZUQ4, TUBA8 and USP18), while the regions flanking HSA22q11.2 on SSC5 correspond to HSA12p13 and HSA12q12. We identified seven distinct chromosomal blocks, further supporting extensive rearrangements between genes on HSA12 and HSA22 in the AMC region on SSC5.  相似文献   

13.
Wang XM  Liu B  Zhao SH  Fan B  Zhu MJ  Yu M  Xiong TA  Li K 《Animal biotechnology》2006,17(1):99-107
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14.
Numerous mapping studies of complex traits in the pig have resulted in quantitative trait loci (QTL) intervals of 10-20 cM. To improve the chances to identify the genes located in such intervals, increased expressed sequence tags (EST)-based marker density, coupled with comparative mapping with species whose genomes have been sequenced such as human and mouse, is the most efficient tool. In this study, we mapped 443 porcine EST with a radiation hybrid (RH) panel (384 had LOD > 6.0) and a somatic cell hybrid panel. Requiring no discrepancy between two-point and multipoint RH data allowed robust assignment of 309 EST, of which most were located on porcine chromosomes (SSC) 1, 4, 7, 8 and X. Moreover, we built framework maps for two chromosomes, SSC1 and SSC7, with mapped QTL in regions with known rearrangement between pig and human genomes. Using the Blast tool, we found orthologies between 407 of the 443 pig cDNA sequences and human genes, or to existing pig genes. Our porcine/human comparative mapping results reveal possible new homologies for SSC1, SSC3, SSC5, SSC6, SSC12 and SSC14 and add markers in synteny breakpoints for chromosome 7.  相似文献   

15.
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16.
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17.
Primary and secondary structure of U8 small nuclear RNA   总被引:20,自引:0,他引:20  
U8 small nuclear RNA is a new, capped, 140 nucleotides long RNA species found in Novikoff hepatoma cells. Its sequence is: m3GpppAmUmCGUCAGGA GGUUAAUCCU UACCUGUCCC UCCUUUCGGA GGGCAGAUAG AAAAUGAUGA UUGGAGCUUG CAUGAUCUGC UGAUUAUAGC AUUUCCGUGU AAUCAGGACC UGACAACAUC CUGAUUGCUU CUAUCUGAUUOH. This RNA is present in approximately 25,000 copies/cell, and it is enriched in nucleolar preparations. Like U1, U2, U4/U6, and U5 RNAs, U8 RNA was also present as a ribonucleoprotein associated with the Sm antigen. The rat U8 RNA was highly homologous (greater than 90%) to a recently characterized 5.4 S RNA from mouse cells infected with spleen focus-forming virus (Kato, N., and Harada, F. (1984) Biochim. Biophys. Acta, 782, 127-131). In addition to the U8 RNA, three other U small nuclear RNAs were found in anti-Sm antibody immunoprecipitates from labeled rat and HeLa cells. Each of these contained a m3GpppAm cap structure; their apparent chain lengths were 60, 130, and 65 nucleotides. These U small nuclear RNAs are designated U7, U9, and U10 RNAs, respectively.  相似文献   

18.
CD9 is a member of the transmembrane-4 superfamily of surface molecules that seems to have a relevant role in cell migration and adhesion, as well as malignant progression. This work describes the isolation of the cDNA coding for the porcine CD9 molecule. Pig CD9 cDNA was isolated from a smooth muscle cDNA library and contains a 678-bp open reading frame with its predicted polypeptide sequence of 226 amino acids. The deduced amino acid sequence conserves the main characteristics of TM4 proteins, including the presence of four transmembrane domains. Like their homologous molecules from other species, pig CD9 has two extracellular regions of a different size with the minor loop bearing two possible glycosylation sites. The pig CD9 gene was localized to chromosome 5q25 by using a somatic cell hybrid panel. Analysis of CD9 expression in different porcine cells and tissues demonstrated that CD9 mRNA is ubiquitously expressed.  相似文献   

19.
Yang K  Ren J  Ma J  Yan X  Huang L 《Biochemical genetics》2007,45(11-12):857-862
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20.
In order to improve the map resolution and to locate more genes on the porcine radiation hybrid map, expressed sequence tags (ESTs) were isolated from a 28-day-old normal pig embryo cDNA library. The ESTs were sequenced from the 5'-end and similarities were checked with sequences registered in the NCBI DNA database (http://www.ncbi.nlm.nih.gov/blast/). The ESTs sequences which have high identity scores (>80%) against human genes or ESTs were further sequenced from the 3' untranslated region. The ESTs which were sequenced successfully were used to design primers for PCR analysis of the radiation hybrid panel. Eleven ESTs were physically mapped to porcine chromosomes 2, 4, 8, 10, 13, 14 and X. The localizations are in agreement with the comparative mapping data between human and pig. The results will provide unique information to the comparative map of human and pig.  相似文献   

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