人类锌指结构新基因ZNF18的克隆和表达谱分析

在很多转录因子中发现的锌指结构,被认为在人类心脏的发育和相关疾病的发生过程中发挥重要的作用。本文报道了克隆和表达分析人类新的锌指蛋白基因ZNF18。该基因cDNA长2 767 bp,编码一个有549个氨基酸的蛋白,这一蛋白含有一个SCAN结构域,一个KRAB结构域和5个连续的C2H2型锌指结构域。ZNF18蛋白与小鼠Zfp535有77％的同源性。ZNF18基因定位于人染色体17p12~p13,包含9个外显子和8个内含子。以ZNF18全长编码区为探针进行Northern杂交,结果显示ZNF18在成体小鼠各组织中广泛表达,但在心脏中低丰度表达。整体原位杂交结果显示,ZNF18基因在小鼠胚胎的表达有很高的动态性。ZNF18主要在E7.5小鼠胚胎的胚外组织表达,E8.5出现了胚胎躯干前端表达。ZNF18从E9.0开始在胚胎的心脏和尾部表达,尤其在E10.5胚胎的心脏高丰度表达。这提示ZNF18基因与心脏发育过程可能有密切的关系。     

人类新基因ZNF418的研究初报

根据计算机克隆的ZNF418基因序列设计引物,从人类胚胎心脏文库中克隆了一个人类新KRAB/C2H2型锌指基因,经国际基因命名委员会批准命名为ZNF418。该基因位于染色体19 q13.43,编码蛋白由676个氨基酸残基组成的、含有1个KRAB框和17个连续排列的C2H2型锌指的蛋白质。Northern杂交的结果表明该基因在多种成人组织中表达;亚细胞定位研究证明ZNF418蛋白主要分布在胞核中。这些结果提示该基因编码一种潜在的转录因子。     

HSVⅠ感染人成纤维细胞诱导的SR-15蛋白生物学功能分析

人单纯疱疹病毒Ⅰ型(HerpessimplexvirusⅠ,HSVⅠ)结合人成纤维细胞相应受体以启动感染的过程,能够引起细胞产生特异性蛋白分子的表达,其中之一的SR-15蛋白经酵母双杂交系统分析证明可与细胞内多个具有KRAB结构的锌指蛋白产生特异性相互作用,其作用部位为锌指结构域,该作用能够影响该类蛋白之一ZNF268在细胞内的转录抑制作用。     

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.     

HSVⅠ感染人成纤维细胞诱导的SR-15蛋白生物学功能分析

人单纯疱疹病毒Ⅰ型(Herpes simplex virusⅠ, HSVⅠ)结合人成纤维细胞相应受体以启动感染的过程,能够引起细胞产生特异性蛋白分子的表达,其中之一的SR-15蛋白经酵母双杂交系统分析证明可与细胞内多个具有KRAB结构的锌指蛋白产生特异性相互作用,其作用部位为锌指结构域,该作用能够影响该类蛋白之一ZNF268在细胞内的转录抑制作用.     

ZNF268基因启动子区的克隆及功能分析

锌指基因家族是人体中最大的基因家族,它参与细胞分化、胚胎发育,并与许多疾病的发生相关。人类ZNF268基因是一个在人胚肝中特异性表达的C2H2型锌指基因,并可能在人的早期肝脏发育中起重要作用。为了研究ZNF268基因表达调控的分子机制,以正常人总基因组为模板PCR扩增了ZNF268基因的5′调控区2533bp片段,并将此片段插入启动子缺失的EGFP(增强型绿色荧光蛋白)载体构建了重组质粒pZNF268—EGFP。用脂质体介导的方法将pZNF268—EGFP转染NIH／3T3、COS7、K562、HeLa4个细胞系。在激光共聚焦显微镜下观察绿色荧光的表达,发现在每个细胞系中,转染了重组质粒pZNF268—EGFP的细胞均有荧光表达,但其起始表达时间均晚于转染了阳性对照质粒pEGFP—C1的细胞且荧光较弱。这表明ZNF268基因的5′调控区2．5kb片段是一个有功能的启动子,但该启动子与CMV启动子相比活性较弱。选择易培养的HeLa细胞系用于缺失研究。将一系列5′端—2456bp至—20bp缺失、3′端均为 77bp的缺失片段插入启动子缺失的CAT(氯酶素酰胺转移酶)载体构建了一系列重组质粒。将这些重组质粒转染HeLa细胞系进行缺失分析,并通过共转染pCMV—Sport—βgal质粒校正转染效率。结果表明,ZNF268启动子—2456～—1639bp区域可能含有正调控元件,—1244～—1013bp和—525～—156bp区域可能含有负调控元件,ZNF268启动子激活转录的一个重要区域位于—156～—20bp。     

pCMV-BD-ZNF424和pCMV-Tag2-ZNF424缺失突变重组质粒的构建

锌指蛋白基因家族是人类最大的基因家族之一,目前已知的很多锌指蛋白成员都是转录调控因子.KRAB/C2H2型锌指蛋白是一类重要的转录因子,ZNF424是该亚家族的一个新成员.已经初步证明ZNF424具有转录激活作用,为了进一步研究ZNF424各结构域激活程度和在信号途径中的作用,设计出引物,以pCMVB-D-ZNF424重组质粒作为模板,PCR扩增出含ZNF424基因的KRAB、LINK和ZNF的3个含不同结构域的区域,克隆到pMD18T-载体,然后内切酶切下各目的片段,再构建出pCMVB-DK-RAB、pCMVB-DL-INK、pCMVB-D-ZNF、pCMVT-ag2BK-RAB、pCMVT-ag2BL-INK和pCMVT-ag2CZ-NF共6个缺失突变重组质粒,为进一步研究ZNF424基因功能奠定基础.     

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。     

哺乳动物锌指蛋白家族中KRAB功能域的进化

KRAB锌指基因是哺乳动物中最大的转录调控因子家族,它的多数成员在基因组上成簇分布,具有五种不同的亚家族,在功能行使上承担着不同的作用。本文通过对人类、黑猩猩、小鼠、大鼠和狗五种哺乳动物全蛋白质组序列及mRNA组织表达谱分析,验证了C2H2锌指结构在单个KRAB蛋白质中出现的数目多于一般锌指蛋白质;KRAB功能域在各物种中分布显著不同且与分化时间不成正比,这表明KRAB相关功能域多样性在灵长类进化过程中潜在的适应性进化。同时,提出KRAB亚家族进化的路线：即KRAB—Aa为起始家族,Ba由Aa直接演变形成,而Ca,blonga和XRCC-Z种亚型可能经过Ba或直接从Aa演变形成;此外,锌指结构在单个蛋白质中出现个数伴随KRAB功能域自身的进化路线逐渐递增,反映了KRAB功能域在形成新转录调控因子方面的积极作用。     

一条KRAB型锌指蛋白全长新基因的克隆与功能初探

从人胎脑cDNA文库中克隆到一条全长的锌指蛋白新基因的cDNA,命名为ZNF303。序列分析表明,ZNF303的C末端含有7个保守的锌指基序,N末端含有一个KRAB(Krüppel?associated box)结构域。利用肝癌组织表达谱基因芯片杂交证明,该基因在肝癌组织中的表达量有明显降低。认为这种降低可能跟肝癌的形成和转移有密切的关系。利用辐射杂交基因定位技术,得出该基因在人类染色体上的位置是19q13.2。 Abstract: We have cloned a full?length novel zinc finger cDNA of the Krüppel family from human fetal brain cDNA library. Sequence analysis indicates that ZNF303 contains 7 highly conserved zinc finger motifs at the C-terminus and a KRAB(Krüppel-associated box)domain at the N-terminus of the deduced rotein.Hybridization using gene chip of hepatic cancer tissue demonstrates the expressive amount in hepatic cancer tissue is lower than control. We hypothecate that the decreasing of expression amount is related to the formation and metastasis of hepatic cancer.Finally,we show that ZNF303 maps on human chromosome 19q13.2 by radiation hybrid.     

Cloning and characterization of a novel Krüppel-like zinc finger gene, ZNF268, expressed in early human embryo

With the aim of identifying genes involved in early human embryonic development, we have isolated a cDNA clone representing a novel human zinc finger gene ZNF268 from 3 week old human embryo cDNA library using a differential hybridization strategy. The complete cDNA sequence of ZNF268 contained an open reading frame of 2841 nucleotides that encodes a 947 amino acid protein with an N-terminal Krüppel-associated box (KRAB) domain and 24 C-terminal zinc fingers. Northern blot analysis showed that ZNF268 mRNA is mainly expressed in 3-5 week old human embryos suggesting it could play certain roles in the embryogenesis. The gene consists of six exons spanning about 22 kb of genomic DNA. According to the genomic sequence from the HTGS database, the ZNF268 gene is assigned to human chromosome 5.     

The Zinc Finger Protein ZNF268 Is Overexpressed in Human Cervical Cancer and Contributes to Tumorigenesis via Enhancing NF-κB Signaling

Cervical cancer is one of the most common tumors affecting women''s health worldwide. Although human papillomavirus can be detected in nearly all cases, the mechanism of cervical carcinogenesis remains to be further addressed. Here, we demonstrated that ZNF268, a Krüppel-associated box-containing zinc finger protein, might contribute to the development of cervical cancer. We found that ZNF268b2, an isoform of ZNF268, was overexpressed in human squamous cervical cancer specimens. Knockdown of ZNF268 in cervical cancer cells caused cell cycle arrest at the G₀/G₁ phase, reduced colony formation, and increased sensitivity to TNFα-induced apoptosis. In addition, HeLa cell growth in xenograft nude mice was suppressed by ZNF268 knockdown, with increased apoptosis. Furthermore, ZNF268b2 was shown to increase NF-κB signaling in vitro and in vivo. Reconstitution of NF-κB activity restored proliferation in ZNF268 knockdown HeLa cells. Of note, we observed a high frequency of NF-κB activation in ZNF268-overexpressing cervical cancer tissues, suggesting a pathological coincidence of ZNF268b2 overexpression and NF-κB activation. Taken together, our results reveal a novel role of ZNF268b2 that contributes to cervical carcinogenesis in part through enhancing NF-κB signaling.     

Molecular cloning and preliminary functional analysis of two novel human KRAB zinc finger proteins, HKr18 and HKr19.

cDNA clones encoding two novel human KRAB zinc finger proteins, HKr18 and HKr19, were isolated from a human testis cDNA library. Their corresponding genes were later identified in sequences originating from chromosomes 19 and 7, respectively. On the basis of the collected information from gene and cDNA sequences, Hkr18 was found to be a protein of 94 kDa with 20 zinc finger motifs in its C terminus. The HKr19 is a smaller protein, with a molecular weight of 56 kDa containing 11 zinc finger motifs. Both HKr18 and HKr19 contained a KRAB A as well as a KRAB B domain in their N termini. Northern blot analysis showed expression of HKr18 in all human tissues tested, indicating a ubiquitous expression pattern. In contrast, HKr19 showed a more restricted tissue distribution, with detectable expression primarily in testis and fetal tissues. The HKr19 protein is a member of the large ZNF91 subfamily of KRAB zinc finger genes. A PCR-based analysis of the expression of HKr19 and other closely related genes showed that lymphoid, myeloid, and nonhematopoietic cells expressed different sets of these genes. This latter finding indicates that some members of the ZNF91 family may be involved in regulating lineage commitment during hematopoietic development. Transfection of various parts of HKr19 into human embryonic kidney cells (HEK 293 cells) showed that the entire protein and its zinc finger region were toxic to these cells when expressed at high levels. In contrast, the KRAB domain and the linker region seemed to be well tolerated.