Molecular Cloning of a Novel Human Acid Phosphatase Gene (ACPT) That Is Highly Expressed in the Testis

Acid phosphatases are enzymes capable of hydrolyzing orthophosphoric acid esters in an acid medium. Prostatic acid phosphatase has served as a tumor marker for metastatic prostate cancer for many years. We have cloned a new human acid phosphatase gene (named testicular acid phosphatase, ACPT), which is expressed mainly in testis and to a lower extent in the prostate, trachea, and other tissues. This gene maps to chromosome 19q13.4, in an area that harbors many cancer-related genes. The testicular acid phosphatase gene is composed of 11 exons, and the protein is predicted to have a luminal domain, a transmembrane domain, and a cytoplasmic domain. The N-terminal end of the protein encodes a signal peptide. The protein has approximately 50% homology with both the prostatic and the lysosomal acid phosphatases, and the position of the cysteine residues, the N-glycosylation sites, and the histidine catalytic site are conserved among the three proteins. The testicular acid phosphatase gene is up-regulated by androgens and is down-regulated by estrogens in the prostate cancer cell line LNCaP. Our preliminary results indicate that this gene exhibits a lower level of expression in testicular cancer tissues than in their normal counterparts.     

一种新型锌指蛋白基因——人ZNF313的克隆、定位及表达(英文 )

运用正常可育男性和无精症病人睾丸组织的mRNA差异显示和cDNA末端快速扩增 (RACE)等方法 ,从人睾丸组织中分离了一个同时含有指环结构和C2 H2 结构域的新型锌指蛋白基因———人ZNF3 13。运用荧光原位杂交 (FISH)方法 ,将该基因定位到人染色体 2 0q13。该基因含 6个外显子 ,编码 2 2 8个氨基酸。基因组结构分析显示 ,外显子 6含有的 2个加尾信号 ,产生 2种不同的 3′端非翻译区。Northern杂交及多组织RT PCR的结果显示该基因含有 0 .75kb和 2 .4kb两种转录本 ,其中0 .75kb转录本在正常睾丸中高表达 ,而其他组织、无精症患者及胎儿睾丸组织中该基因低表达。结果提示 :人ZNF3 13基因对精子发生和男性可育性可能起重要作用     

Cloning and Characterization of a Gene (RFN22) Encoding a Novel Brain Expressed Ring Finger Protein (BERP) That Maps to Human Chromosome 11p15.5

We have recently identified a novel RING finger protein expressed in the rat brain, which associates with myosin V and α-actinin-4. Here we have cloned and characterized the orthologous human BERP cDNA and gene (HGMW-approved symbol RNF22). The human BERP protein is encoded by 11 exons ranging in size from 71 to 733 bp, and fluorescence in situ hybridization shows that the BERP gene maps to chromosome 11p15.5, 3′ to the FE65 gene. The human BERP protein is 98% identical to the rat and mouse proteins, and we have identified a highly conserved potential orthologue in Caenorhabditis elegans. BERP belongs to the RING finger–B-box–coiled coil (RBCC) subgroup of RING finger proteins, and a cluster of these RBCC protein genes is present in chromosome 11p15. Chromosome region 11p15 is thought to harbor tumor suppressor genes, and deletions of this region occur frequently in several types of human cancers. These observations indicate that BERP may be a novel tumor suppressor gene.     

运用数字差异展示方法克隆一个人类新的锌指蛋白基因ZNF474

运用数字差异展示方法,克隆一个与生精相关的睾丸高表达基因。借助公共ESTs数据库,利用DDD软件比较分析各种睾丸文库与其他组织或细胞系文库有差异表达的ESTs,成功克隆到一个在人类睾丸中高表达的新基因。结合实验获得新基因cDNA全长,该基因被国际人类基因命名委员会命名为ZNF474(GeneBank登陆号AY461732)。ZNF474的cDNA全长为1 972 bp,定位在5 q23.2。通过RT-PCR及测序验证,其开放阅读框的位置在377 bp~1 471 bp处,编码364个氨基酸,在氨基酸水平与小鼠同源基因有66%的一致性,而与其他已知蛋白质无明显同源性。Northern杂交分析显示ZNF474在成体睾丸组织特异高表达,卵巢组织弱表达,在多种其他组织中不表达,为单一转录本。原位杂交显示ZNF474基因在正常成人睾丸组织各级生精细胞、隐睾组织以及精原细胞癌组织中均有较高表达。综上考虑,推测ZNF474作为生殖细胞中特异的转录因子,对人类的精子发生和卵母细胞的发育可能起重要作用。     

一个新的人类锌指蛋白基因ZNF474的cDNA克隆和表达分析

数据库消减杂交就是利用NCBI中的Unigene数据库中大量的数据资源,收集各种细胞或组织的基因表达谱进行两两比较或多重比较,获得两组文库间有统计学意义的差异表达基因。运用NCBI中的数据库消减杂交分析方法,从人睾丸组织中分离了一个含有C2H2结构的新型锌指蛋白基因-ZNF474(GenBank登录号：AY461732)．通过推导和进一步的RT—PCR实验证实：该基因含2个外显子,gDNA在染色体上跨度30065bp,定位于人染色体5q23．1-q23。2．cDNA编码一个含364个氨基酸的新蛋白,分子质量是40．3kDa,等电点为9．59。Northem杂交结果显示：该基因含有2．37kb大小的唯一转录本,主要在睾丸中很强表达,卵巢中有弱表达,而其他组织中该基因无表达．结果提示：ZNF474基因对精子发生和卵母细胞的发育可能起重要作用、     

小鼠BTB/锌指结构新基因Bsg6的克隆及表达谱分析

Bsg6 (brain specific gene 6) 是用消减差异筛选的方法克隆的小鼠头部特异表达 新基因. Bsg6基因cDNA长3 871 bp,编码一个670个氨基酸残基的蛋白,GenBank 登录号AY635051,位于小鼠第4号染色体,由2个外显子构成. Bsg6蛋白含有一个N端BTB（Broad complex, Tramtrack, and Bric a brac）结构域和两个C端C２Ｈ２型锌指结构域. 小鼠Bsg6蛋白与其在人类和鸡中同源蛋白的同源性分别为86.2%和79.1%. Bsg6在小鼠胚胎中的表达具有一定动态性,在E8.5的小鼠胚胎中,Bsg6主要在前脑和神经管表达. 在E9.5的小鼠胚胎中,Bsg6的表达明显增强并主要集中在前脑的端脑部. Bsg6在E10.5小鼠胚胎端脑的表达出现了下降,但是在中脑和后脑的表达增加,此外,Bsg6 mRNA的表达还出现在肢芽和尾部. 在HH10期的鸡胚中,Bsg6主要在头部和神经管前端表达. Northern杂交结果显示,Bsg6在很多小鼠成体组织中没有表达,但是在破骨细胞瘤中高表达. Bsg6的表达谱提示,Bsg6可能是在器官形成期对脑的发育起到重要作用的转录因子,而且其表达受到严格的调控,此外Bsg6还能与肿瘤的发生有关.     

在人类胚胎发育过程中表达的新锌指蛋白基因ZNF359的研究

kriipple型锌指蛋白是一类具有重要功能的转录调节因子。初步克隆了一个新的人类kriipple型锌指蛋白基因,经国际基因命名委员会批准命名为ZNF359。此基因长3271个碱基,含6个外显子,在基因组DNA上长18kb。它编码的蛋白质全长643个氨基酸,含一个KRAB框,16个C2H2型的锌指,在两者之间还有一个典型的中间重复序列。Northern Bolt分析表明该基因在人类早期胚胎的各个组织中普遍表达,且在肾、心脏和肺的表达水平最强。其结构和表达特征预示着它编码的是一个具DNA结合功能的转录调控因子。     

小鼠睾丸和卵巢特异表达基因Zfp474的克隆与特征分析

运用NCBI中的数据库消减杂交(Digital Differential Display,DDD)分析方法,从小鼠睾丸组织中分离了一个含有C2HC／C3H结构的新型锌指蛋白基因——ZIM74(GenBank登录号：AY350709)。通过推导和进一步的RT-PCR实验证实：该基因含4个外显子,gDNA在染色体上跨度29869bp,定位于小鼠染色体18D1。cDNA编码一个含347个氨基酸的新蛋白,带有C2HC／C3H结构域。Northern杂交结果显示：该基因含有2．37kb大小的唯一转录本,主要在睾丸中强表达,卵巢中有表达,而在其他组织中该基因无表达。结果提示：Zfp474基因对精于发生和卵母细胞的发育可能起重要作用。     

人类锌指蛋白ZNF382对肌生成的调控作用

人类基因组中有大量哺乳类特有的KRAB锌指基因,这些基因的功能大多尚不清楚,ZNF382就是其中一个.本文研究了人类锌指蛋白ZNF382对肌生成的调控作用.人类ZNF382基因在肌肉组织中高表达,ZNF382的mRNA水平在C2C12细胞的肌生成过程中上调,ZNF382调节肌肉特异性基因的表达,在NIH3T3细胞中,ZNF382与E-box蛋白E12和成肌调节因子MyoD共转增强肌肉肌酸激酶MCK启动子的活性;ZNF382的启动子预测分析也发现ZNF382的启动子上含有MyoD和血清反应因子SRF的结合位点,这些结果提示人类ZNF382蛋白在肌生成中起着重要的作用.     

一个小鼠睾丸特异表达新基因mtIQ2的克隆和表达谱分析

运用数据库消减杂交筛选出一个在小鼠睾丸中特异表达的新基因--mtIQ2 (Genbank Accession No: DQ153247), Northern blot结果表明该基因的cDNA序列全长为1.2kb,小鼠多组织RT-PCR结果表明:该基因在睾丸中特异表达,而在其他组织中没有表达.运用隐睾模型对该基因的表达研究表明:在手术后第9d,该基因表达急剧下降,到18d完全消失.这些实验提示该基因在睾丸的发育和性成熟过程中可能起重要作用.     

A Novel Zebrafish Gene Expressed Specifically in the Photoreceptor Cells of the Retina

We have identified and characterized a novel protein from adult zebrafish retina, which we named ES1. Database search revealed that the ES1 gene has significant similarity to two genes with unknown functions: theEscherichia colisigma cross-reacting protein 27a (scrp27a) and the human KNP-I/GT335.In situhybridization and immunohistochemistry experiments showed that both ES1 mRNA and protein are expressed specifically in adult photoreceptor cells. ES1 seems to be a cytoplasmic protein. An ES1-like antigen was also detected in photoreceptor cells of goldfish with anti-ES1 antibodies. The retina specific expression and the evolutionary conservation suggest that ES1 protein may be important for maintaining normal retina structure and function.     

The Zinc Finger Protein Zfr1p Is Localized Specifically to Conjugation Junction and Required for Sexual Development in Tetrahymena thermophila

Conjugation in Tetrahymena thermophila involves a developmental program consisting of three prezygotic nuclear divisions, pronuclear exchange and fusion, and postzygotic and exconjugant stages. The conjugation junction structure appears during the initiation of conjugation development, and disappears during the exconjugant stage. Many structural and functional proteins are involved in the establishment and maintenance of the junction structure in T. thermophila. In the present study, a zinc finger protein-encoding gene ZFR1 was found to be expressed specifically during conjugation and to localize specifically to the conjugation junction region. Truncated Zfr1p localized at the plasma membrane in ordered arrays and decorated Golgi apparatus located adjacent to basal body. The N-terminal zinc finger and C-terminal hydrophobic domains of Zfr1p were found to be required for its specific conjugation junction localization. Conjugation development of ZFR1 somatic knockout cells was aborted at the pronuclear exchange and fusion conjugation stages. Furthermore, Zfr1p was found to be important for conjugation junction stability during the prezygotic nuclear division stage. Taken together, our data reveal that Zfr1p is required for the stability and integrity of the conjugation junction structure and essential for the sexual life cycle of the Tetrahymena cell.     

A Novel Zinc Finger Protein 219-like (ZNF219L) is Involved in the Regulation of Collagen Type 2 Alpha 1a (col2a1a) Gene Expression in Zebrafish Notochord

The notochord is required for body plan patterning in vertebrates, and defects in notochord development during embryogenesis can lead to diseases affecting the adult. It is therefore important to elucidate the gene regulatory mechanism underlying notochord formation. In this study, we cloned the zebrafish zinc finger 219-like (ZNF219L) based on mammalian ZNF219, which contains nine C2H2-type zinc finger domains. Through whole-mount in situ hybridization, we found that znf219L mRNA is mainly expressed in the zebrafish midbrain-hindbrain boundary, hindbrain, and notochord during development. The znf219L morpholino knockdown caused partial abnormal notochord phenotype and reduced expression of endogenous col2a1a in the notochord specifically. In addition, ZNF219L could recognize binding sites with GGGGG motifs and trigger augmented activity of the col2a1a promoter in a luciferase assay. Furthermore, in vitro binding experiments revealed that ZNF219L recognizes the GGGGG motifs in the promoter region of the zebrafish col2a1a gene through its sixth and ninth zinc finger domains. Taken together, our results reveal that ZNF219L is involved in regulating the expression of col2a1a in zebrafish notochord specifically.