端粒结合蛋白TRF2的研究进展

端粒DNA结合蛋白TRF2(TTAGGG repeat binding factor-2)以二聚体形式通过Myb结构域与端粒重复序列TTAGGG结合,并与TRF1、TIN2、Rap1、TINT1及POT1蛋白组成Shelterin蛋白复合物,协同在端粒动态平衡维持过程中起关键作用,进而影响整个基因组的稳定性。此外,TRF2在细胞DNA损伤应答过程中可能发挥重要作用。本文将对TRF2结构和功能研究的最新进展进行综述。     

DNA端粒控制的解密

维持基因组完整性是每个生物生存的关键 ,端粒保护是维持这一稳定的重要机制之一。体内有多种蛋白复合物共同作用以保证DNA末端不丢失或染色体末端不发生融合。端粒酶和其它一些蛋白在维持端粒的过程中有重要作用 ,这些蛋白如何共同维持端粒的正确长度并在细胞分裂过程中复制端粒是一个复杂的机制。Loayza等发现 ,人体内的POT1是一种与酵母细胞中结合单链端粒DNA蛋白相关的蛋白。POT1分子出现在人染色体的末端 ,而且POT1出现在染色体末端的量与多鸟嘌呤核苷酸单链重复区域多少有关 ,重复区域越多 ,POT1出现的越多。POT1不是完全靠…     

端粒保护蛋白

端粒保护蛋白（pmtection of telomere 1,PoT1）是存在于人和裂殖酵母的端粒相关蛋白,特异性地与端粒单链DNA相结合。人POT1基因位于7号染色体上,由22个外显子组成,其中4个外显子属于跳跃外显子,可形成5个剪接变异体。POT1的功能在于维持端粒的稳定,通过TRF1．TIN2．PIP1-POT通路调节端粒长度。     

端粒保护蛋白1(POT1)的研究进展

端粒保护蛋白1(protection of telomeres 1,POT1)几乎存在于所有真核生物中,是一种高度保守表达的蛋白质,它与一系列相关的端粒结合蛋白共同参与保护端粒的结构和功能。随着近年来研究的深入,POT1与端粒的结合特点以及保护端粒的机制有了进一步的完善。此外,POT1对端粒长度的调节方式以及与肿瘤的发生、发展和细胞凋亡等关系也呈现出多样化。结合近几年的研究文献,对POT1的功能以及与其它相关蛋白的作用加以综述。     

一种含有端粒重复序列非编码RNA的发现及最新研究进展

端粒是染色体末端的特化结构,由简单呈串联线性排列的核酸重复序列及相关蛋白质组成。其核酸序列具有高度的保守性,均富含GC。在人类为TTAGGG的高度重复序列具有维持基因组完整性的作用。端粒功能异常会导致染色体失去稳定性,促进肿瘤的发生和发展。以往认为端粒附近区域不具有转录活性,但最近在Science杂志上Azzalin等首次报道了该区域可以转录一种非编码RNA,即端粒RNA(telomeric RNA)。该分子具有特殊的UUAGGG重复序列,在调控端粒长度和端粒酶活性上具有重要作用,在发育、衰老和肿瘤发生发展等研究中已成为热点。该文将对近期有关端粒RNA的研究进展予以综述。     

端粒、端粒酶结构功能研究进展

端粒是真核生物线性染色体末端由重复DNA序列和蛋白质结合形成的复合结构,其特殊的环形结构与多种结合蛋白形成了端粒的多重功能的基础。端粒的功能包括染色体末端的保护、引导减数分裂的同源染色体配对、参与DNA修复过程等;端粒酶具有逆转录酶特性和维持端粒长度的功能,其活性与恶性肿瘤的发生密切相关,调控因子错综复杂。     

果蝇限制端粒转座子的分子机制

端粒是保护线性染色体末端的核酸-蛋白复合物。与常见的真核生物短重复序列组成的端粒不同,黑腹果蝇(Drosophila melanogaster)端粒DNA由反转座子组成,其转座行为被果蝇宿主严格限制在端粒,既实现延长端粒的功能,也减少转座子跳跃对基因组的损伤。但果蝇宿主是如何完成如此精确调控的机制尚不明确。目前已知的全基因组范围抑制转座子表达包括H3K9me3参与的异染色质形成途径和piRNA路径,而近期研究发现果蝇端粒保护蛋白参与端粒反转座子的特异调控。本文主要综述了端粒保护蛋白在调控端粒转座子中的具体功能。对果蝇端粒转座子调控的研究有利于更好地理解宿主与转座子协同进化的分子机制。     

流式原位荧光杂交——测定端粒长度

端粒是染色体末端ＤＮＡ重复序列与特异结合蛋白的复合体。脊椎动物端粒重复序列是 5′ＴＴＡＧＧＧ3′。端粒长度可以作为细胞的“分裂时钟” ,反映细胞的分裂能力。作为染色体末端的帽状结构 ,端粒还有其他生物学功能 :保证染色体完整性 ,使真正的遗传信息得到完整复制 ;保护染色体末端 ,防止染色体异常重组而影响细胞分裂 ;指导染色体与核膜相接。端粒 端粒酶系统对细胞增殖、细胞衰老、细胞永生化、癌变、发育生物学、ＨＩＶ感染的免疫反应、免疫缺陷等有重要意义[1～ 3] 。因此端粒动力学的研究十分重要。1 .ＤＮＡ印迹杂交端粒长度测…     

染色体端粒研究进展

染色体端粒(telomere)是真核生物线性染色体两端的特殊DNA--蛋白质复合体结构,由随机重复序列组成的DNA序列和与之相结合的蛋白质分子构成。端粒DNA无论在DNA顺序、功能及其特殊的复制方式都与其它DNA顺序显著不同。本文将近年来对端粒的DNA结构、与端粒DNA相结合的蛋白质分子和在端粒复制中起重要作用的反转录酶--端粒酶(telomerase)的研究进展以及端粒对于真核生物的重要作用作一综述。     

端粒结合蛋白与端粒长度调节

端粒结合蛋白与端粒长度调节郑晓飞王升启孙志贤（军事医学科学院放射医学研究所,北京１００８５０）关键词端粒端粒结合蛋白端粒是真核细胞染色体的末端序列,其功能是保持染色体的稳定性。端粒ＤＮＡ的长短和稳定性决定了细胞的寿命,并与细胞的癌变和衰老有关。端粒Ｄ...     

Human POT1 facilitates telomere elongation by telomerase

Mammalian telomeric DNA is mostly composed of double-stranded 5'-TTAGGG-3' repeats and ends with a single-stranded 3' overhang. Telomeric proteins stabilize the telomere by protecting the overhang from degradation or by remodeling the telomere into a T loop structure. Telomerase is a ribonucleoprotein that synthesizes new telomeric DNA. In budding yeast, other proteins, such as Cdc13p, that may help maintain the telomere end by regulating the recruitment or local activity of telomerase have been identified. Pot1 is a single-stranded telomeric DNA binding protein first identified in fission yeast, where it was shown to protect telomeres from degradation [10]. Human POT1 (hPOT1) protein is known to bind specifically to the G-rich telomere strand. We now show that hPOT1 can act as a telomerase-dependent, positive regulator of telomere length. Three splice variants of hPOT1 were overexpressed in a telomerase-positive human cell line. All three variants lengthened telomeres, and splice variant 1 was the most effective. hPOT1 was unable to lengthen the telomeres of telomerase-negative cells unless telomerase activity was induced. These data suggest that a normal function of hPOT1 is to facilitate telomere elongation by telomerase.     

Multiple hPOT1–TPP1 cooperatively unfold contiguous telomeric G-quadruplexes proceeding from 3′ toward 5′, a feature due to a 3′-end binding preference and to structuring of telomeric DNA

Telomeres are DNA repeated sequences that associate with shelterin proteins and protect the ends of eukaryotic chromosomes. Human telomeres are composed of 5′TTAGGG repeats and ends with a 3′ single-stranded tail, called G-overhang, that can be specifically bound by the shelterin protein hPOT1 (human Protection of Telomeres 1). In vitro studies have shown that the telomeric G-strand can fold into stable contiguous G-quadruplexes (G4). In the present study we investigated how hPOT1, in complex with its shelterin partner TPP1, binds to telomeric sequences structured into contiguous G4 in potassium solutions. We observed that binding of multiple hPOT1–TPP1 preferentially proceeds from 3′ toward 5′. We explain this directionality in terms of two factors: (i) the preference of hPOT1–TPP1 for the binding site situated at the 3′ end of a telomeric sequence and (ii) the cooperative binding displayed by hPOT1–TPP1 in potassium. By comparing binding in K⁺ and in Li⁺, we demonstrate that this cooperative behaviour does not stem from protein-protein interactions, but from structuring of the telomeric DNA substrate into contiguous G4 in potassium. Our study suggests that POT1-TPP1, in physiological conditions, might preferentially cover the telomeric G-overhang starting from the 3′-end and proceeding toward 5′.     

POT1 proteins in green algae and land plants: DNA-binding properties and evidence of co-evolution with telomeric DNA

Telomeric DNA terminates with a single-stranded 3′ G-overhang that in vertebrates and fission yeast is bound by POT1 (Protection Of Telomeres). However, no in vitro telomeric DNA binding is associated with Arabidopsis POT1 paralogs. To further investigate POT1–DNA interaction in plants, we cloned POT1 genes from 11 plant species representing major branches of plant kingdom. Telomeric DNA binding was associated with POT1 proteins from the green alga Ostreococcus lucimarinus and two flowering plants, maize and Asparagus. Site-directed mutagenesis revealed that several residues critical for telomeric DNA recognition in vertebrates are functionally conserved in plant POT1 proteins. However, the plant proteins varied in their minimal DNA-binding sites and nucleotide recognition properties. Green alga POT1 exhibited a strong preference for the canonical plant telomere repeat sequence TTTAGGG with no detectable binding to hexanucleotide telomere repeat TTAGGG found in vertebrates and some plants, including Asparagus. In contrast, POT1 proteins from maize and Asparagus bound TTAGGG repeats with only slightly reduced affinity relative to the TTTAGGG sequence. We conclude that the nucleic acid binding site in plant POT1 proteins is evolving rapidly, and that the recent acquisition of TTAGGG telomere repeats in Asparagus appears to have co-evolved with changes in POT1 DNA sequence recognition.     

hnRNP A2/B1 binds specifically to single stranded vertebrate telomeric repeat TTAGGGn.

We have previously isolated a protein from mouse liver nuclei that specifically binds to single stranded (TTAGGG)n repeats. TTAGGG is the telomeric repeats of mammals and we therefore named the new protein single stranded telomere binding protein (sTBP). Further studies now identify sTBP as heterogeneous nuclear ribonucleoprotein (hnRNP) A2/B1 on the basis of amino acid sequence determination and antibody reactivity. A2 and B1 form a major part of the protein component of hnRNP particles and are abundant nuclear proteins. Unexpectedly, A2/B1 has a high specificity for binding to the RNA equivalent of TTAGGG, UUAGGG, but under the same conditions does not appear to have a strong affinity for a number of other RNA species.     

Suppression of hPOT1 in diploid human cells results in an hTERT-dependent alteration of telomere length dynamics

POT1 is a 3' telomeric single-stranded overhang binding protein that has been implicated in chromosome end protection, the regulation of telomerase function, and defining the 5' chromosome terminus. In human cancer cells that exhibit constitutive hTERT activity, hPOT1 exerts control over telomere length. Primary human fibroblasts express low levels of catalytically active hTERT in an S-phase-restricted manner that fails to counteract telomere attrition with cell division. Here, we show that diploid human fibroblasts in which hPOT1 expression has been suppressed harbor telomeres that are longer than control cells. This difference in telomere length delays the onset of replicative senescence and is dependent on S-phase-restricted hTERT expression. These findings are consistent with the view that hPOT1 promotes a nonextendable telomere state resistant to extension by S-phase-restricted telomerase. Manipulating this function of hPOT1 may thus hasten the cytotoxic effects of telomerase inhibition.     

ST-1, a 39-kilodalton protein in Trypanosoma brucei, exhibits a dual affinity for the duplex form of the 29-base-pair subtelomeric repeat and its C-rich strand.

In our attempt to identify telomere region-binding proteins in Trypanosoma brucei, we identified ST-1, a polypeptide with novel features. ST-1 was chromatographically purified from S-100 cell extracts and was renatured from a sodium dodecyl sulfate-protein gel as a 39-kDa polypeptide. It forms a specific complex with the trypanosome telomere repeats of TTAGGG, but more significantly, it shows a higher affinity for the 29-bp subtelomere repeats of T. brucei. These 29-mer boxes are a large tandem series of telomere-derived repeats which separate the simple telomere DNA from middle-repetitive telomere-associated sequences on many chromosomes. ST-1 is the first example of a protein binding within such large repetitive subtelomere elements in trypanosomes or other organisms. ST-1 is also novel in that it has a selective affinity for the C-rich strands of both the subtelomeric 29-mer and the telomere repeats, comparable to that for the duplex form of the respective repeats. All previously described telomere-binding proteins have affinity for only the duplex form or for the G-rich strand. This C-rich strand binding specificity of ST-1 may provide insight into this protein's mechanism of binding in vivo.     

DNA binding features of human POT1: a nonamer 5'-TAGGGTTAG-3' minimal binding site, sequence specificity, and internal binding to multimeric sites

The human telomeric protein POT1 is known to bind single-stranded telomeric DNA in vitro and to participate in the regulation of telomere maintenance by telomerase in vivo. We examined the in vitro DNA binding features of POT1. We report that deleting the oligosaccharide/oligonucleotide-binding fold of POT1 abrogates its DNA binding activity. The minimal binding site (MBS) for POT1 was found to be the telomeric nonamer 5'-TAGGGTTAG-3', and the optimal substrate is [TTAGGG](n (n > or = 2)). POT1 displays exceptional sequence specificity when binding to MBS, tolerating changes only at position 7 (T7A). Whereas POT1 binding to MBS or [TTAGGG](2) was enhanced by the proximity of a 3' end, POT1 was able to bind to a [TTAGGG](5) array when positioned internally. These data indicate that POT1 has a strong sequence preference for the human telomeric repeat tract and predict that POT1 can bind both the 3' telomeric overhang and the displaced TTAGGG repeats at the base of the t-loop.     

A TRF1-controlled common fragile site containing interstitial telomeric sequences

Mouse telomeres have been suggested to resemble common fragile sites (CFS), showing disrupted TTAGGG fluorescent in situ hybridization signals after aphidicolin treatment. This “fragile” telomere phenotype is induced by deletion of TRF1, a shelterin protein that binds telomeric DNA and promotes efficient replication of the telomeric ds[TTAGGG]n tracts. Here we show that the chromosome-internal TTAGGG repeats present at human chromosome 2q14 form an aphidicolin-induced CFS. TRF1 binds to and stabilizes CFS 2q14 but does not affect other CFS, establishing 2q14 as the first CFS controlled by a sequence-specific DNA binding protein. The data show that telomeric DNA is inherently fragile regardless of its genomic position and imply that CFS can be caused by a specific DNA sequence.     

Sequence-specific DNA recognition by the myb-like domain of the human telomere binding protein TRF1: a model for the protein-DNA complex.

Telomeres consist of tandem arrays of short G-rich sequence motifs packaged by specific DNA binding proteins. In humans the double-stranded telomeric TTAGGG repeats are specifically bound by TRF1 and TRF2. Although telomere binding proteins from evolutionarily distant species are not sequence homologues, they share a Myb-like DNA binding motif. Here we have used gel retardation, primer extension and DNase I footprinting analyses to define the binding site of the isolated Myb-like domain of TRF1 and present a three-dimensional model for its interaction with human telomeric DNA. Our results suggest that the Myb-like domain of TRF1 recognizes a binding site centred on the sequence GGGTTA and that its DNA binding mode is similar to that of the homeodomain-like motifs of the yeast telomere binding protein RAP1. The implications of these findings for recognition of telomeric DNA in general are discussed.