不同品种实验兔虹膜酪氨酸酶基因序列和表达量的变化

目的从酪氨酸酶基因序列和表达量两个方面探讨酪氨酸酶与家兔虹膜颜色表型的关系。方法通过PCR扩增和测序检测4个具有不同颜色性状的家兔品种的酪氨酸酶基因外显子序列多态性;通过荧光定量PCR检测酪氨酸酶基因表达水平。结果白化品种日本大耳白兔和獭兔的TYR基因序列在第1118个碱基处都由C突变为A,并导致编码蛋白在373位,即最后一个N-糖基化位点发生由Thr到Lys的突变。白毛黑眼兔和青紫兰兔在第870个碱基处全部发生由A到T的无义突变。在白毛黑眼兔种群的所有个体和獭兔种群的部分个体中都发现TYR基因序列在第91个碱基处发生G到A的突变,导致氨基酸序列第31位处Val到Met的变异。经内参基因GAPDH的校正,TYR基因在白毛黑眼兔和青紫兰兔中表达水平显著高于在日本大耳白兔和獭兔中的表达水平（P〈0.01）。而在白毛黑眼兔和青紫兰兔之间、日本大耳白兔和獭兔之间,TYR基因的表达差异没有显著性。结论家兔TYR基因突变可能大幅度降低TYR基因表达,导致酪氨酸酶功能低下,从而影响虹膜颜色表型。     

白毛黑眼兔黑眼性状的遗传模式

目的揭示白毛黑眼兔黑眼性状的遗传模式。方法选取具有黑眼突变性状的白毛黑眼兔与其背景品系日本大耳白兔进行杂交,构建6个两代杂交家系。对杂交产生的F1代和F2代个体虹膜颜色性状的观察和统计,并应用遗传数理统计方法中常用的分离分析进行遗传模式探讨。结果χ2检验显示,杂交实验所得虹膜颜色分布的观察值与常染色体单基因显性遗传模式的期望值差异无显著性(P0.05),与常染色体隐性遗传及伴性遗传模式的期望值差异有显著性(P0.05)。结论白毛黑眼兔的黑眼突变是由常染色体上单个基因的变异造成的显性性状。     

白毛黑眼兔等四种实验兔黑色素分布的组织学观察与比较

目的：分析包括白毛黑眼兔在内的四个品种实验兔的虹膜和皮肤组织中的黑色素分布情况和相互之间的差异。方法通过组织切片和硫酸亚铁染色,对四个品种实验兔的虹膜和皮肤组织中的黑色素含量和分布进行了观察与比较。结果与其背景白化品种相比,白毛黑眼兔不仅在虹膜组织中出现了类型完整的黑色素,而且在其表型为白色的皮肤的毛囊中也出现了低含量的黑色素。结论本结果为白毛黑眼兔突变表型机理研究提供了一定线索。     

二化螟β1微管蛋白基因cDNA序列的克隆与序列分析

微管是真核生物体内分布最为广泛的一类蛋白,是由a-和β-两种不同的微管蛋白组成的异源二聚体.微管参与许多细胞功能,如细胞形态发生、细胞生长和分裂等.以二化螟3龄幼虫为材料提取总RNA,利用RT-PCR和cDNA末端快速扩增技术(RACE),扩增得到该虫的β微管蛋白基因的cDNA序列一条.cDNA序列含1 862个碱基,开放读码框1 344个碱基,编码氨基酸447个,分子量约为50.2kD,等电点4.82.氨基酸序列中1～4个氨基酸MREI为β微管蛋白转录后调控信号,是微管蛋白特异片段;氨基酸序列的140～146GGGTGSG位存在一个微管蛋白标志信号片段.序列比对表明,克隆的β微管蛋白基因与其他昆虫的β微管蛋白基因在核苷酸和氨基酸水平上都是高度同源的,与家蚕Bombyx moriβ1微管蛋白的氨基酸序列同源性达到99.1%,与烟草天蛾β1微管蛋白的氨基酸序列同源性达到98.7%,与果蝇Drosophila melanogasterβ1微管蛋白的氨基酸序列同源性达到96.9%.该基因cDNA序列已经登录Genbank并获得登录号为EU429675.     

小鼠脂联素受体2基因编码区的克隆及序列分析

构建小鼠脂联素受体2(mAdipoR2)基因cDNA克隆,并进行序列及基因结构分析,为进一步研究小鼠AdipoR2的表达和生物学活性奠定基础。用RT—PCR方法扩增mAdipoR2基因cDNA,获得的片段连接至pGEM-T载体,转化JM109大肠杆菌,经酶切鉴定后,进行序列测定。利用因特网生物信息学资源分析mAdipoR2基因序列。结果成功地构建了mAdipoR2基因cDNA克隆,其序列与GenBank登录序列一致。通过与小鼠基因组序列比对,分析了mAdipoR2基因结构,其编码序列由7个外显子组成,编码1个含7个跨膜区的膜蛋白,但该受体不属于G蛋白偶联受体家族(GPCRs)。mAdipoR2与人及大鼠蛋白的同源性分别为91％和95％。     

人、猴、兔BPI活性部位基因的克隆和序列分析

为比较不同动物来源杀菌／通透性增加蛋白（BPI）的活性部位在基因组成上的差异,为今后对人BPI进行分子改构打下基础,分别从人、恒河猴和家兔外周血白细胞中克隆出BPI全长或活性部位基因,进行序列分析和比较,并进行蛋白二级结构预测。结果发现：猴、兔BPI活性部位序列与人序列在核苷酸水平的同源性分别为94％和77％,在氨基酸水平的同源性分别为88％和62％;人氨基酸序列中包含一个糖基化位点,而猴、兔序列没有;兔序列比人、猴序列少一个氨基酸;3种BPI活性部位有近似的二级结构。     

基于CRISPR/Cas9技术构建Plin1基因敲除小鼠模型及表型分析

利用CRISPR/Cas9技术构建纯合围脂滴蛋白(Plin1)基因敲除小鼠模型,并初步分析其表型.针对Plin1基因2号外显子前后序列设计sgRNA并构建表达载体,体外转录获得sgRNA后与Cas9蛋白混合,显微注射至小鼠受精卵中并进行胚胎移植.出生小鼠经测序及PCR基因型鉴定获得Fo代阳性小鼠;令Fo代小鼠与野生型小...     

新生小鼠兴奋性氨基酸转运蛋白家族成员cDNA的克隆和分析

兴奋性氨基酸转运蛋白家族包含几种结构相似的膜蛋白,它们在终止谷氨酸的突触传递作用,维持神经系统正常的递质水平起重要作用.为了在同一物种中研究这些蛋白和基因的功能,本工作对新生小鼠脑的兴奋性氨基酸转运蛋白家族成员进行了克隆,获得了3个谷氨酸转运蛋白亚型(mGLAST-1,mGLT-1,mEAAC1)和一个中性氨基酸转运蛋白(mASCT1)的cDNA,其中在小鼠中mASCT1序列为首次发表.序列分析表明,mASCT1cDNA的长度为3787bp,编码一个532个氨基酸箴基的蛋白,和人的ASCT1蛋白序列有89.3%的同源性,用非洲爪蟾卵母细胞表达系统证实了它具有转运丝氨酸的活性.同时,我们的研究表明,兴奋性氨基酸转运蛋白mRNA的5'UTR和3'UTR普遍存在组成和长度的不均一性,这种现象可能提示该家族成员的基因表达具有转录后调控机制.     

猪POU1F1基因部分序列变异和同源性分析

对长白、杜洛克、约克夏、姜曲海、梅山和香猪等六个猪种的POU1F1基因第四、第五和第六外显子分别进行PCR扩增,并对含有第四、第六外显子的PCR产物和含有第五外显子的克隆产物进行测序。结果表明：六个猪种中,POU1F1基因的第四外显子存在碱基突变,为T→C。对该序列进行Nla Ⅲ 酶消化,产生两种不同的基因型(GG和HH);而第五和第六外显子则高度保守,未发现任何突变。将人POU1F1基因第四外显子、POU同源区核苷酸编码序列和氨基酸序列,分别与猪、小鼠、牛的POU1F1基因相应的核苷酸序列和氨基酸序列进行同源性比较,结果发现：人与猪、小鼠、牛的POU1F1基因第四外显子的核苷酸同源性分别高达93.9%、86.7%、92.1%,而由第四外显子编码的部分POU特异区的氨基酸序列则完全一致;人与猪、小鼠、牛POU同源区的核苷酸同源性分别为91.4%、85.1%、87.9%,氨基酸同源性分别为96.6%、94.8%、90.2%。这说明在哺乳动物中,其POU1F1蛋白的POU同源区和由第四外显子编码的POU特异区部分是高度保守的;猪可作为实验动物,建立人类相关疾病模型,为医学研究提供参考依据。     

异源四倍体鲫鲤及其原始父母本细胞周期蛋白B基因克隆与分子遗传分析

细胞周期蛋白(cyclin)B是真核细胞周期运转中调控G2期至M期转化的关键因子.本实验根据斑马鱼细胞周期蛋白 B1基因的剪切方式,设计3对特异于金鱼和银鲫细胞周期蛋白B基因外显子区兼并引物,首次扩增出异源四倍体鲫鲤及其原始亲本红鲫和鲤鱼细胞周期蛋白B基因2条大小分别约为2.4 kb和2.1 kb的片段.测序及比对分析表明：这3种鱼的细胞周期蛋白B基因2个片段均包含8个外显子和7个内含子.内含子剪切位点符合GT/AG规则,推测细胞周期蛋白B基因2个片段可能是细胞周期蛋白B基因的2种存在形式.异源四倍体鲫鲤与其原始父母本细胞周期蛋白B基因片段序列的比较结果表明：无论是外显子区还是内含子区,异源四倍体鲫鲤与其原始亲本都具有较高的遗传相似性,在1 025 bp的外显子序列中相同的碱基位点数达963个,为异源四倍体鲫鲤来源于红鲫和鲤鱼提供了分子证据;同时,异源四倍体鲫鲤与其原始亲本差异碱基位点的存在又表明这一独特的多倍体物种与其原始亲本存在着进化上的变异.此外,还分别以细胞周期蛋白B基因外显子和内含子序列构建了包括异源四倍体鲫鲤及其原始父母本在内的系统进化树.结果初步表明：对于亲缘关系较近的物种,用外显子和内含子序列构建的系统进化树与传统的物种进化树一致;而对于亲缘关系较远的物种,用内含子序列构建的进化树与传统的物种进化顺序存在较大差异.     

The human homolog of the mouse brown gene maps to the short arm of chromosome 9 and extends the known region of homology with mouse chromosome 4.

The mouse brown locus encodes a tyrosinase-related protein, TRP-1. The human homolog of TRP-1 was recently cloned from a melanoma cDNA library and sequenced. We have made oligonucleotide primers corresponding to the human TRP1 3' untranslated region and used them to map the human TRP1 gene by species-specific PCR in human/rodent somatic cell hybrids. By this means, the human TRP1 gene has been mapped to the short arm of chromosome 9.     

Cloning and characterization of the rabbit POU5F1 gene.

The product of the POUSF1 gene, Oct4, plays an important role both in embryonic development and in the self-renewal and differentiation of totipotent cells. To understand the function of Oct4 in rabbit ES cells, we cloned and sequenced the rabbit POU5F1 gene, as well as the cDNA encoded by the gene. The Oct4 cDNA contains a 1083 bp ORF encoding a 360 aa protein and a 241 bp 3' UTR sequence. Oct4 mRNA was expressed at a high level in rabbit ES cells and was barely detectable in the adult spleen, kidney, brain and muscle tissues. The POU5F1 gene is approximately 6 kb in length and includes five exons and four introns. Gene organization is similar to that of the mouse, human and bovine orthologs. Sequencing of the gene revealed an 82% (mouse), 90% (human) and 89% (bovine) overall identity at the protein level. The rabbit POUSF1 gene was mapped to chromosome 12q1.1 by PCR amplification of DNA from two putative POU5F1-containing BAC clones, which were previously mapped to chromosome 12q1.1. The cloning of the rabbit POU5F1 gene will facilitate studies on its roles in rabbit embryogenesis and ES cells.     

Cloning and sequencing of cDNA coding for rabbit alpha-1-antiproteinase F: amino acid sequence comparison of alpha-1-antiproteinases of six mammals

Rabbit liver cDNA coding for alpha-1-antiproteinase F has been isolated and sequenced. The protein sequence deduced from the nucleotide sequence consists of a 24 amino acid signal peptide and 389 amino acids of the mature polypeptide. Rabbit alpha-1-antiproteinase F showed 74 and 64% homology to human alpha-1-antiproteinase at the nucleotide and amino acid levels, respectively, but the N-terminal five amino acids are lacking in the rabbit protein. The sequences of alpha-1-antiproteinase F of rabbit, human, baboon, sheep, rat, and mouse show about 40% identity, and the reactive site (Met-Ser) is conserved. On the other hand, variable regions are located in the second half to the C-terminal as well as in the N-terminal region.     

Sequence and expression of human protein kinase C-epsilon.

Two human homologues of protein kinase C-epsilon (E1 and E2) were isolated from two distinct cDNA libraries. Sequence comparisons to PKC-epsilon cDNAs from several species indicated that each of these human epsilon clones contained cloning artifacts. Thus, a composite PKC-epsilon (E3) clone was derived from clones E1 and E2. Human PKC-epsilon (E3) has an overall sequence identity of 90-92% at the nucleotide level compared to the previously characterized mouse, rat and rabbit clones. At the amino acid level, the deduced human epsilon sequence shows a 98-99% identity with the mouse, rat and rabbit sequences. Expression of the human PKC-epsilon clone in Sf9 cells confirmed that the recombinant protein displayed protein kinase C activity and phorbol ester binding activity. The recombinant protein was also recognized by two distinct epsilon-specific polyclonal antibodies.     

Mouse liver cytochrome P-450 (P-450IIIAM1): its cDNA cloning and inducibility by dexamethasone.

A full-length cDNA complementary to mouse liver mRNA coding for one of the cytochromes P-450 (P-450) in the P-450IIIA family, namely P-450IIIM1, was isolated and completely sequenced. The sequence of this cDNA clone, pMDex13, revealed that it encoded a polypeptide of 504 deduced amino acid residues (Mr = 57,853). The deduced amino acid sequence showed 87.3 and 84.9% identity with rat P-450IIIA1 and P-450IIIA2, respectively. The NH2-terminal 24 amino acid sequences of P-450IIIAM1 were completely identical with purified mouse P-450UT protein. RNA blot analysis showed that mRNA content of hepatic P-450IIIAM1 was remarkably increased by treatment of mice with dexamethasone.     

家兔BMP7基因的克隆及其生物信息学分析

在对已知部分编码序列(CDS)进行分析的基础上, 采用RT-PCR分步扩增以及RACE方法, 对家兔BMP7基因3′和5′末端未知序列进行了克隆与生物信息学分析。测序结果综合分析表明, 所获序列共计1 654 bp, 包括家兔BMP7近全长前肽、全长成熟肽CDS及3′非翻译序列(3′UTR), 将已有的序列向5′和3′端分别延伸了395 bp和628 bp。序列对比表明, 克隆的家兔BMP7 CDS部分与人、小鼠的对应序列的同源性分别为91.89%和89.32%, 预测的氨基酸序列同源性分别为96.51%和96.01%。家兔BMP7 3′UTR长446 bp, 与人、小鼠对应序列同源性分别为57.38%和45.57%; 具有2个转录终止信号位点。推测家兔BMP7成熟蛋白有BMPs特有的7个位置固定的半胱氨酸残基和TGF-β家族指纹。家兔BMP7 3′UTR区转录终止信号的可选择性可能与基因转录后调控有关。     

cDNA cloning of human oxysterol-binding protein and localization of the gene to human chromosome 11 and mouse chromosome 19

Cellular cholesterol metabolism is regulated primarily through sterol-mediated feedback suppression of the activity of the low-density lipoprotein receptor and several enzymes of the cholesterol biosynthetic pathway. We previously described the cloning of a rabbit cDNA for the oxysterol-binding protein (OSBP), a cytosolic protein of 809 amino acids that may participate in these regulatory events. We now use the rabbit OSBP cDNA to clone the human OSBP cDNA and 5' genomic region. Comparison of the human and rabbit OSBP sequences revealed a remarkably high degree of conservation. The cDNA sequence in the coding region showed 94% identity between the two species, and the predicted amino acid sequence showed 98% identity. The human cDNA was used to determine the chromosomal localization of the OSBP gene by Southern blot hybridization to panels of somatic cell hybrid clones containing subsets of human or mouse chromosomes and by RFLP analysis of recombinant inbred mouse strains. The OSBP locus mapped to the long arm of human chromosome 11 and the proximal end of mouse chromosome 19. Along with previously mapped genes including Ly-1 and CD20, OSBP defines a new conserved syntenic group on the long arm of chromosome 11 in the human and the proximal end of chromosome 19 in the mouse.     

Characterization of the 46,000-dalton subunit of eIF-4F

Three protein synthesis initiation factors, eukaryotic initiation factor (eIF)-4A, -4B, and -4F are required for the ATP-dependent binding of mRNA to the ribosome. To extend the characterization of the eIF-4A-like subunit of eIF-4F, a cDNA clone encoding eIF-4A has been isolated from a rabbit liver cDNA library and sequenced. The clone is almost full length for the coding region and complete for the 3' noncoding region. The sequence of the rabbit cDNA has been compared to the sequence of the two similar, but not identical, genes and cDNAs encoding mouse eIF-4A (termed eIF-4AI and eIF-4AII). The rabbit cDNA sequence is very similar to the mouse eIF-4AI genomic and liver cDNA sequence with 100% identity at the amino acid level and 90% identity at the nucleotide level within the protein coding region; however, there is very little similarity in the 3' noncoding region. Amino acid sequencing of purified rabbit reticulocyte eIF-4A protein indicates that it is eIF-4AI (encoded by the eIF-4AI gene and cDNA) and none of the amino acid residues sequenced are in disagreement with those predicted from the mouse liver or rabbit liver cDNA sequences. Subsequently, we have analyzed the p46 subunit of eIF-4F, a three subunit protein whose molecular weights have been estimated by sodium dodecyl sulfate gel electrophoresis to be 220,000, 46,000 and 24,000. The p46 subunit has physical properties similar to eIF-4A. This subunit was isolated from rabbit reticulocyte eIF-4F and sequenced chemically. Our results indicate that this peptide is a mixture of eIF-4AI and eIF-4AII in an approximate ratio of 4 to 1, respectively. No eIF-4AII was observed in our rabbit reticulocyte eIF-4A preparation. Therefore we have concluded that either the eIF-4AI and the eIF-4AII proteins were resolved from each other in the purification of rabbit reticulocyte eIF-4A or that eIF-4AII preferentially associates with the p220 and p24 subunits of eIF-4F. Evidence favoring the latter possibility is discussed.     

一种新的短链脱氢/还原酶家族新成员:NADP(H)-依赖的视黄醇脱氢酶基因的克隆和分析

从牛的肝脏中快速抽提总RNA,根据GenBank已发表NADP(H)-依赖的视黄醇脱氢酶基因(NRDR)的cDNA序列,设计并合成特异引物,利用cDNA末端快速扩增(RACE)方法和反转录-聚合酶链式反应(RT-PCR),得到牛肝内的NRDR cDNA的全长序列。经测序证实,牛肝NRDR的全长cDNA序列为1266bp,其开放读码框架在24～806bp,编码260个氨基酸(GenBank登录号：AF487454)。根据NRDR基因推导出的氨基酸序列与人、鼠、兔有高度同源性,并含有SDR超家族成员的两个高度保守的模序,在其C-端含有过氧化物酶体的靶向序列为SHL。结果表明,牛的NRDR应属于过氧化物酶体内SDR超家族成员并在维甲酸合成的限速步骤起作用的酶,也为维甲酸合成的传统通路提供一个补充。