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Molecular cloning of the canine c-Met/HGF receptor and its expression in normal and regenerated liver 总被引:4,自引:0,他引:4
Neo S Kansaku N Furuichi M Watanabe M Hisamatsu S Ohno K Hisasue M Tsuchiya R Yamada T 《The Journal of veterinary medical science / the Japanese Society of Veterinary Science》2005,67(5):525-529
The c-Met proto-oncogene is the receptor for hepatocyte growth factor (HGF), which is a member of the tyrosine kinase family. Activation of the HGF/c-Met signal pathway leads to cell proliferation, motility, regeneration, and morphogenesis. In this study, the complete nucleotide sequence of complementary DNA (cDNA) of canine c-Met was cloned, and its distribution was determined in tissues. The canine c-Met cDNA clone had an open reading frame of 4419 bp that encoded a putative polypeptide of 1383 amino acids. The c-Met mRNA was expressed in a variety of canine tissues including peripheral blood mononuclear cells (PBMC), bone marrow, liver, kidney, lung, stomach, uterus, testis, thymus, lymph node, small intestine, colon, adrenal gland, thyroid gland, heart, muscle, skin, pancreas, ovary, prostate, spleen, fat, cerebrum, and cerebellum. In addition, the c-Met mRNA expression in normal and regenerated liver was examined. The levels of the mRNA increased 2-fold in regenerated liver compared to that found in normal liver, indicating that c-Met is involved in various functions including remodeling of canine hepatocytes. 相似文献
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Full-length canine HSP70 cDNA was sequenced and the expression of HSP70 mRNA was investigated. The full-length cDNA sequence of the HSP70 gene (2322 bp) contained a single long open reading frame (1920 bp) coding a protein of 640 amino acids. The amino acid sequence of the canine HSP70 gene shared about 90-95% sequence similarity with bovine, human and mouse HSP70 proteins. Southern blot analysis with HSP70 probe gave three distinct bands of 9.4 kb, 5 kb and 4.4 kb in BamHI digests and two distinct bands of 19 kb and 4 kb in EcoRI digests. Canine HSP70 mRNA was detectable in canine peripheral blood mononuclear cells and stomach but not in liver, kidney, spleen, small intestine, large intestine and skin of dogs. 相似文献
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Cloning and analysis of a novel cDNA from Trichinella spiralis encoding a protein with an FYVE zinc finger domain 总被引:2,自引:0,他引:2
Fu BQ Liu MY Kapel CM Meng XP Lu Q Wu XP Chen QJ Boireau P 《Veterinary parasitology》2005,132(1-2):27-30
A cDNA library from Trichinella spiralis adults 3 days post-infection was screened with a cDNA probe, designated T 54, derived from a newborn larvae subtracted cDNA library. Sequence analysis showed that the positive clone contained a cDNA insert of 1464 bp in length with a single open reading frame of 1290 bp, which encoded a protein of 429 amino acids with a putative molecular mass of 49.9 k Da. Database analysis predicted the deduced protein had a leucine zipper motif and an FYVE zinc finger domain. The recombinant fusion protein was expressed and rabbit anti-recombinant protein sera reacted with a single peptide migrating at approximately 55 k Da in crude worm extract from muscle larvae, adults and newborn larvae stages. 相似文献
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旋毛虫新生幼虫WN1抗原基因的克隆及表达 总被引:1,自引:0,他引:1
应用旋毛虫人工感染猪血清对旋毛虫新生幼虫cDNA文库进行免疫筛选,对阳性克隆WN1序列进行生物信息学分析。结果表明,WN1 cDNA全长为474bp,含有1个354bp的完整的开放阅读框架(ORF),编码的多肽由117个氨基酸残基组成,其相对分子质量理论推导值为13200,等电点为4.25,N-末端的信号肽表明其可能为分泌性蛋白。GenBank数据库检索结果显示,此序列为一个新基因的全长cDNA。经PCR扩增WN1基因,将其克隆到原核表达载体pET28a,重组质粒经鉴定后,转化大肠杆菌BL21 star(DE3)并诱导表达出相对分子质量为15000的重组蛋白,与理论设计完全相符。 相似文献
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根据GenBank已收录的牛(Bos taurus)、人(Homo sapiens)和小鼠(Mus musculus)等物种Ets-1基因序列的同源保守区域,设计特异性引物,采用RT-PCR和RACE技术,分离并克隆了西农萨能奶山羊(Capra hircus)Ets-1基因的cDNA序列。该序列全长2 263 bp(GenBank登录号HQ589338),包括5’UTR 331 bp,CDS 1 326bp和3’UTR 606 bp,编码441个氨基酸组成的蛋白质。核苷酸序列分析发现,山羊编码序列与牛、猪、人、小鼠等的相应序列同源性分别为98%、94%、92%和90%,3’UTR相应序列为96%、83%、81%和77%,5’UTR相应序列为98%、85%、82%和71%。氨基酸序列分析发现,山羊与牛、猪、人和小鼠的Ets-1的相似性较高,均在95%以上。蛋白质结构分析发现,其蛋白质分子量为50 340.8 D,等电点为5.08,具有典型的螺旋-转角-螺旋结构域,不存在跨膜结构,并且整个序列不含信号肽。 相似文献
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WRKY 转录因子家族在植物生长发育各个阶段发挥重要作用。本研究运用电子克隆和RT-PCR 结合的方法获得1个紫花苜蓿WRKY 转录因子家族成员的cDNA 序列,命名为MsWRKY56。该序列长1267bp,包含1个951bp的最大开放阅读框,编码317个氨基酸;构建该基因的瞬时表达载体,通过基因枪轰击洋葱表皮的方法对编码蛋白进行亚细胞定位研究,结果表明该基因编码蛋白定位于细胞核,符合转录因子的亚细胞定位特征,为进一步研究该基因编码蛋白的结构和功能奠定了基础。 相似文献
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Okamura Y Ma Z Khatlani TS Okuda M Une S Nakaichi M Taura Y 《The Journal of veterinary medical science / the Japanese Society of Veterinary Science》2003,65(8):913-915
Receptor-binding cancer antigen expressed on SiSo cells (RCAS1) is a novel cancer cell-surface antigen, strongly expressed in invasive cancers. RCAS1 inhibited the in vitro growth of immunocytes, and induced apoptotic cell death. The cloning of canine RCAS1 cDNA was carried out and identified from the mammary gland tumor of a dog. A canine RCAS1 cDNA of 864 bp in length has an open reading frame of 642 bp nucleotides encoding a protein of 213 deduced amino acids. The predicted amino acid sequence of canine RCAS1 showed 96.2% and 96.7% homologies with those of human and mouse RCAS1 respectively. Canine RCAS1 has an N-terminal transmembrane segment and a coiled-coil structure in the C-terminal protein, which are highly conserved in mouse and human RCAS1. 相似文献
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旋毛虫新生幼虫期特异性T314全长cDNA的克隆及表达 总被引:4,自引:1,他引:3
利用PCR将旋毛虫新生幼虫期特异性全长T314cDNA的信号肽祛作后重组到原核表达载体pET-28a。将重组质粒pET28-T314转入克隆菌DH5a和表达菌DE3,分别提取质粒进行酶切,测序鉴定。用KIPTG诱导培养重组表达菌DE3,做菌体裂解物外源表达产物的SDS-PAGE分析。将重组质粒表达的融合蛋白免疫家兔制备抗血清,采用Western blot检测T314cDNA在旋毛虫不同发育时期的表达情况及其天然表达产物的相对分子质量。测序结果显示:外源T314cDNA的PCR产物在重组质粒pET28-T314中阅读框架正确;SDS-PAGE分析结果显示:经IPTG诱导后转化菌DE3的裂解产物与对照菌相比出现了1条相对分子质量约为39000的新条带,大小与外源cDNA融合蛋白的理论推导值38800相符;Western blot检测结果显示:T314cDNA的天然表达产物仅存在旋毛虫新生幼虫,不存在于成虫与肌幼虫,且相对分子质量大小与其在原核重组质粒中表达产物相同。 相似文献
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应用旋毛虫感染猪血清,对旋毛虫新生幼虫cDNA文库进行了免疫筛选。对阳性克隆pBK-cMV-WN10的序列分析结果表明。cDNA全长为1352bp。含有1个1218bp的完整的开放阅读框架(ORF),编码的多肽由406个氨基酸残基组成,其相对分子质量理论推导值为45900,等电点为5.43,N末端的信号肽及糖基化位点(NCS)表明其可能为分泌性糖蛋白,氨基酸序列19~156与158~295为重复区域,相似性为74%.C末端有1个半胱氨酸蛋白酶抑制剂结构域,但旋毛虫p46000抗原与其他线虫的半胱氨酸蛋白酶抑制蛋白结构有很大差异,可能已经失去半胱氨酸蛋白酶抑制蛋白的功能。PCR结果显示。从旋毛虫新生幼虫、肌幼虫、3日龄成虫和5日龄成虫cDNA中均扩增出此基因,表明此基因在旋毛虫各个时期均有表达。 相似文献
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Yamazaki J Hasebe N Nagafuchi S Baba K Tsujimoto H Kano R Hasegawa A 《Veterinary microbiology》2004,101(1):1-8
In the present study, full length of feline bax, bcl-2, bcl-xL and caspase 3 genes were sequenced and the expression of these mRNAs were also investigated in FIV-infected lymphocytes. The full length cDNA sequence of bax (646 bp), bcl-2 (1423 bp), bcl-xL (1163 bp) and caspase 3 genes (1208 bp) contained a single open reading frame of 579 bp coding 193 amino acids, 708 bp coding 236 amino acids, 702 bp coding 234 amino acids and 834 bp coding 278 amino acids, respectively. Number of apoptotic Kumi-1 cells gradually increased after FIV infection and approximately 70% were apoptotic and 30% were viable in the cells infected with FIV after 8-day incubation, though approximately 80% were non-apoptotic and 20% were dead in non-infected cells. The expression of bcl-2 mRNA in lymphocytes of established cell line was increased by FIV. The amounts of mRNAs of bax, caspase 3 and bcl-xL in FIV-infected cells were not different from those in uninfected control cells. 相似文献
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为了研究不同泌乳期乳腺组织中差异表达基因,利用抑制性削减杂交技术构建西农萨能羊泌乳60d乳腺组织及泌乳28d乳腺组织中差异表达基因文库,用Real-Time PCR技术验证阳性克隆血清淀粉样蛋白A3(SAA3)基因,通过RT-PCR方法克隆西农萨能羊乳腺组织SAA3,并进行序列比对和功能预测。结果成功构建了西农萨能羊不同泌乳期乳腺组织中差异表达基因文库,筛选克隆了乳腺组织SAA3基因,GenBank登录号为:DQ839400,编码区长度为396bp,含有131个氨基酸。西农萨能羊乳腺组织中SAA3与牛(GenBank:NM_181016)、兔(GenBank:M64696.1)、人(GenBank:BC020795)、鼠(GenBank:NM_011315)核苷酸同源性分别为95%、84.3%、81.3%和81.9%,氨基酸同源性为93%、76%、72%、72%;在编码区261-287位较人、兔、鼠SAA编码区多27个碱基,连续大于5个氨基酸的保守区域有6个,较人SAA多3个潜在功能基序。 相似文献
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体节极性基因dpp是昆虫发育过程中的关键基因。采用生物信息学的方法,利用家蚕EST数据获得了家蚕dpp基因(Bmdpp)cDNA序列。该cDNA序列全长1 206 bp,ORF1 146 bp,编码381个氨基酸,预测蛋白分子质量38.6 kD,等电点9.18。将克隆的Bmdpp基因完整CDS序列亚克隆到pET-28a(+)表达载体,转化、诱导后经SDS-PAGE电泳检测到约40 kD与预测分子质量相符的目的蛋白条带。对Bmdpp在家蚕胚胎不同发育时期的表达分析发现,该基因在受精6~14 h的表达量很低,甚至没有表达。这一表达模式和果蝇dpp基因在胚胎发育过程中的表达模式相似,推测Bmdpp在家蚕早期胚胎发育的背-腹轴分化中起作用。 相似文献
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采用SMART RACE 方法,从东方山羊豆盐诱导抑制性差减杂交cDNA 文库中分离到了一个脱水蛋白(GoDHN)基因。该基因cDNA 全长1169bp,开放阅读框843bp,编码281 个氨基酸,编码的蛋白质分子量为28.71kDa。经实时荧光定量PCR 分析,GoDHN 基因在东方山羊豆的茎和叶中表达量明显高于根中表达量,并且基因表达受ABA、NaCl和PEG 的诱导,随着诱导时间的增加,表达量呈持续增长趋势。这些结果表明,DHN 基因在东方山羊豆的抗逆性中可能起到重要的调控作用。本研究成功构建了pCAMBIA1302-DHN 植物表达载体,为下一步转基因研究奠定了基础。 相似文献
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本研究旨在克隆牦牛酪蛋白基因家族(CSN1S1、CSN1S2、CSN2和CSN3)的CDS区序列,鉴定其在牦牛不同组织中的表达水平。选取4岁龄左右处于泌乳期的健康类乌齐母牦牛3头,屠宰后分别采集乳腺、心脏、肝脏、骨骼肌组织,分别提取组织总RNA并反转录为cDNA,设计酪蛋白基因家族特异性引物扩增酪蛋白基因家族序列,进行生物信息学分析,并利用实时荧光定量PCR法分别检测酪蛋白家族基因mRNA水平。结果显示,克隆得到CSN1S1、CSN1S2、CSN2和CSN3基因cDNA序列分别为919、832、805和715bp,其CDS区全长分别为645、669、690和585bp,分别编码214、222、259和194个氨基酸残基。类乌齐牦牛酪蛋白基因家族与黄牛亲缘关系最近,其次是印度水牛,而与单胃动物猪的亲缘关系最远。组织表达结果显示,酪蛋白基因家族在组织中广泛表达,其中在乳腺组织中的表达量最高,其次是骨骼肌组织。在乳腺组织中CSN1S1、CSN1S2、CSN2基因之间表达量差异不显著(P>0.05),但CSN2基因表达量显著高于CSN3基因(P<0.05)。以上结果为酪蛋白基因家族在牦牛乳腺蛋白质代谢调控机制的研究提供了参考依据。 相似文献
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ZHANG Hao ZHAO Jia-ping WU Qiong YANG Ying DU Zhan-yu GUO Yue-yue XING Xiu-mei XU Chao ZHANG Lin-bo 《中国畜牧兽医》2016,43(10):2527-2533
To in-depth analyze the molecular structure characteristics of agouti gene,using bioinformatic methods for RNA-Seqs test to get the complete coding sequence of raccoon dog agouti gene,and its coding protein structure was forecasted and analyzed.The results showed that the length of raccoon dog agouti gene cDNA was 530 bp which contained 396 bp open reading frame (ORF),encoded 131 amino acids.Predicting the weight of the raccoon dog agouti protein molecular was 14.41 ku and isoelectric point (pI) was 9.68,as the unstable hydrophohbic protein;It contained 11 phosphorylation sites,1 glycosylation sites and a long reach 24 amino acid signal peptide;Random coil was the main secondary structure.Phylogenetic tree showed that the raccoon dog had a close genetics distance to vuipe and canis familiaris which was consistent with the traditional animal taxonomy.Through the analysis of the molecular structure characteristics of raccoon dog agouti gene,to provide the oretical basis for revealing the influence of the colour diversity molecular genetics mechanism. 相似文献
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本试验以鲤鱼外周血白细胞肿瘤坏死因子受体相关因子6(tumor necrosis factor receptor-associated factor 6,TRAF6)EST序列为基础,经地高辛标记后作为探针,对有丝分裂原刺激的鲤鱼外周血白细胞cDNA文库进行核酸杂交筛选,从重组噬菌体中经过两轮筛选获得阳性克隆。序列分析结果显示,该序列包含有5'-非编码区(5'-UTR) 25 bp;3'-非编码区(3'-UTR) 535 bp,存在2个mRNA不稳定基序ATTTA;开放阅读框ORF长1632 bp,编码543个氨基酸。预测蛋白质等电点为5.88,分子质量大小为61.773 ku。序列同源性比对结果表明,所获得的序列与GenBank上登录的鲤鱼TRAF6a基因同源性达99%。蛋白质序列分析结果发现,其具有TRAF家族的典型序列特征。 相似文献
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Wang Z Petersen K Weaver MS Magnuson NS 《Veterinary immunology and immunopathology》2001,78(2):177-195
The cDNA clone of bovine pim-1 has been isolated from phorbol-12-myristate-13-acetate (PMA) and concanavalin A (ConA)-activated peripheral blood lymphocytes (PBLs). The full-length cDNA contains a 411bp 5' untranslated region (5'-UTR), followed by a 939bp coding region and a 3' untranslated region (3'-UTR) that contains 1403bp. Comparison of the bovine pim-1 coding sequence with the human, rat, mouse, frog and zebrafish counterparts reveals 94, 90, 89, 67 and 40% homology at the nucleotide level, respectively. The predicted amino acid sequence of bovine Pim-1 shares 98.7, 97.1, 93.3, 68.8, and 52.4% similarity with the sequences of human, rat, mouse, frog, and zebrafish, respectively. The 5'-UTR of bovine pim-1 shares high sequence similarity to the human and mouse counterparts and is G/C-rich (75%) which may promote a high degree of secondary structure. The 3'-UTR of bovine pim-1 contains two potential polyadenylation sites and an A/T-rich motif which has been shown to decrease the stability of polyA mRNA molecules. Southern blot results indicate that a single copy of the gene exists in the bovine genome. Northern blot results show that PMA stimulation of PBLs increases the expression of the pim-1 mRNA. In addition, examination of Pim-1 protein expression in PBLs stimulated with a variety of mitogens including ConA, PMA, anti-CD3 and purified protein derivative (PPD) from Mycobacterium tuberculosis, reveals two different types of expression patterns during the course of a 24h period of stimulation. ConA and PPD gave a biphasic pattern of expression while PMA and anti-CD3 gave single transient pattern of expression suggesting that expression is controlled by more than one signaling pathway. 相似文献