ABC转运蛋白结构及在植物病原真菌中的功能研究进展

ABC(ATP-binding cassette)转运蛋白是最大的膜转运蛋白超家族之一,其主要功能是利用ATP水解产生的能量将底物进行逆浓度梯度运输.所有生物体都含有大量ABC蛋白.ABC蛋白位于细胞的不同空间,如细胞膜、液泡、线粒体和过氧化物酶体.通常,ABC转运蛋白由跨膜结构域(TMD)和核苷酸结合结构域(NBD)组成,分别与底物和ATP结合.NBD执行与ATP结合和水解,是ABC转运蛋白的动力引擎,TMD识别特异性配体.大多数ABC转运蛋白最初是通过研究生物体耐药性而被发现的,包括多效耐药(PDR)和多药耐药(MDR).本文对ABC转运蛋白的结构及作用机制,以及植物病原真菌中ABC转运蛋白功能的研究进展进行综述.     

植物ABC和MATE转运蛋白与次生代谢物跨膜转运

植物产生大量的次生代谢物,不但对植物自身适应性具有极其重要的作用,而且有着巨大的实用价值。次生代谢物的跨膜转运是植物次生代谢工程研究的一个新兴领域。ABC（ATP-binding cassette）和MATE（multidrug and toxin extrusion）转运蛋白与生物体内多种物质的跨膜转运有关,在植物次生代谢物的运输过程中均发挥着重要作用。文章主要综述了ABC和MATE转运蛋白在植物次生代谢物跨膜转运中的研究进展。     

植物ABCB转运蛋白研究进展

ABC转运蛋白家族是一类通过结合并水解ATP释放能量实现底物的跨膜运输的转运蛋白,它们参与了植物众多的生理代谢过程,根据保守区的进化关系将ABC转运蛋白家族分成8个亚族,其中ABCB转运蛋白为第二大亚族。ABCB 转运蛋白具保守的NBDs结构域,由6个跨膜α-螺旋的疏水跨膜结构域组成了TMDs结构域,形成溶质跨膜的通道,但是其结构、长度与序列则变化多样。按分子大小不同将植物ABCB转运蛋白分为全分子转运蛋白、半分子转运蛋白两类,通过测序发现在拟南芥、水稻和番茄等植物上均有一定比列的ABCB转运蛋白,且行使多种功能。有研究表明,ABCB转运蛋白基因介导镉、铅和铝等重金属离子的转运,提高植物重金属耐性;它直接参与植物体内生长素的运输,从而调控植物高度;它还可能将苹果酸从质体转运到保卫细胞中调节气孔的开合。近年来,越来越多的ABCB转运蛋白被鉴定,但是ABCB亚家族庞大,底物特异性强,转运机制复杂,多数转运蛋白的功能尚未确定。因此,了解ABCB转运蛋白在生命活动过程中的重要性,以及基因表达调控的机制,解析ABCB转运蛋白在响应逆境胁迫过程中的重要作用,以期为植物抗逆性育种提供思路。     

酸性土壤上植物应对铝胁迫的过程与机制

铝胁迫是酸性土壤上影响作物产量最重要的因素之一.目前,全球土壤酸化程度进一步加剧了铝胁迫.植物可通过将铝离子与有机酸螯合储藏于液泡和从根系中排出铝毒.排出铝毒主要通过苹果酸转运蛋白ALMT和柠檬酸转运蛋白MATE的跨膜运输来实现.编码ABC转运蛋白和锌指转录因子的基因与植物抗铝胁迫有关.这些抗铝毒基因的鉴别使得通过转基因和分子标记辅助育种等生物技术来提高农作物的抗铝毒能力成为可能.最后提出了植物抗铝胁迫研究中需要解决的关键问题及今后的研究方向.     

植物PDR蛋白转运机制及功能的研究进展

植物多向耐药性（pleiotropic drug resistance,PDR）基因亚家族是ATP结合盒（ATP-binding cassette,ABC）基因家族的一员,其编码的PDR蛋白通过水解ATP释放能量、引起蛋白构象变化实现物质跨膜转运。PDR蛋白可以转运萜类物质、植物生长素和金属离子以应答外界生物和非生物胁迫。综述植物PDR蛋白结构、转运机制及其功能,为克隆植物PDR基因并深入研究其结构与功能提供基础知识。     

拟南芥ABC转运类蛋白家族的分子进化、表达模式和蛋白功能网络预测分析

ABC转运蛋白又称腺苷三磷酸结合盒转运蛋白(ATP-binding cassette transporters),该基因家族是目前已知最大、最古老的蛋白家族之一,在植物中ABC转运蛋白种类繁多、结构复杂、功能多样,涉及植物一切的生命活动过程。本研究系统介绍了拟南芥中131个ABC转运蛋白的亚家族分类、系统命名、蛋白大小以及蛋白亚细胞定位等基因信息,在此基础上,分析了ABC转运蛋白基因在染色体分布以及进化过程中发生的复制事件;其次在47个组织器官或发育阶段中聚类分析了ABC转运蛋白的表达模式和各个亚家族分布规律,结果表明ABC转运蛋白基因的表达具有明显的组织特异性和时空特异性,说明在进化过程中该类蛋白功能也进一步发生分化;我们以花药发育过程为例,说明ABC转运蛋白在花药发育过程中具有较高的协调性,在时空和组织上表达受到严格的调控;最后我们分析了ABC转运蛋白亚家族内部和各个亚家族之间可能存在的蛋白相互作用关系,推测ABC半分子转运蛋白形成同源或异源二聚体发挥功能的可能性,进一步说明ABC转运蛋白在蛋白互作水平上也存在功能多样性和严格的调控关系。     

不同生物土壤结皮微生物组跨膜转运蛋白基因多样性及差异

【背景】跨膜转运蛋白在微生物转运各种物质的过程中具有重要作用。【目的】通过比较原核微生物组磷酸转移酶(phosphotransferasesystem,PTS)系统和腺苷三磷酸结合盒(ATP-binding cassette,ABC)转运蛋白编码基因在两种不同生物土壤结皮中(藻结皮与藓结皮)的差异,以期揭示随着生物土壤结皮的发育演替,微生物组跨膜转运物质的生物学过程中的潜在变化趋势。【方法】对腾格里沙漠东南缘的藻结皮和藓结皮12个样品进行宏基因组测序,参照KEGG数据库PTS系统,与ABC转运蛋白代谢通路进行比较并筛选相关基因,分析其差异显著性。【结果】藻结皮和藓结皮PTS系统和ABC转运蛋白编码基因的多样性一致。在生物土壤结皮中共检测到16种PTS系统的转运蛋白的编码基因,具有显著性差异的有5种;检测到106种ABC转运蛋白的编码基因,具有显著性差异的有46种,并对这46种转运蛋白结合的底物以及变化趋势进行了详细的描述。【结论】生物土壤结皮发育演替过程中,微生物组从环境中摄取能够增加渗透势物质的潜力总体呈现降低趋势,转运氨基酸、细胞膜和细胞壁组分的潜力总体呈现增加趋势,对于矿物离子、辅助因子、糖类和碳酸氢盐等的转运潜力总体无明显变化。需要注意的是这些转运蛋白编码基因多样性及差异与生物土壤结皮的关系还有待实验证明与解释。     

结核分枝杆菌ABC转运蛋白与物质的跨膜转运

结核分枝杆菌作为一种胞内寄生菌,主要存在于巨噬细胞吞噬体内,并且通过与宿主细胞竞争摄取营养物质、主动排出有毒物质来维持生存。因此,参与上述过程的ABC转运蛋白在结核分枝杆菌的致病中发挥着举足轻重的作用。已有报道结核分枝杆菌基因组编码了38个ABC转运蛋白。这类蛋白质有着广泛的底物结合谱,参与了无机离子、糖类、氨基酸、寡肽、药物等多种物质的跨膜转运。本文将对结核分枝杆菌编码的ABC转运蛋白超家族中的不同成员及其底物特异性、转运机制以及与毒力的关系的研究进展进行综述。     

植物Na+/H+反向转运蛋白的研究进展

盐胁迫是限制植物生长发育的主要因素之一,植物Na+/H+反向转运蛋白可通过将Na+逆向转运出细胞外或将Na+区隔化于液泡中来抵制环境中过高的Na+浓度.植物中Na+/H+反向转运蛋白存在于细胞质膜和液泡膜上,现在已得到多种编码这些Na+/H+反向转运蛋白的基因,对其结构功能特性进行了大量研究,并发现将这些基因转入非抗盐植物中过量表达可提高转基因植物的抗盐性.概述了Na+/H+反向转运蛋白及其编码基因的最新研究进展.     

植物ABCB亚家族生物学功能研究进展

ABC转运蛋白超家族结构和功能复杂多样, 包含ABCA-ABCH八个亚家族。ABCB是ABC转运蛋白的一个亚家族, 多数定位于质膜, 少数定位于线粒体膜或叶绿体膜。ABCB与其它生长素转运蛋白(AUX1/LAX、PIN)共同参与调控植物生长素的极性运输, 在植物生长发育的各个阶段发挥作用。此外, ABCB转运蛋白还调控植物的向性运动和重金属抗性等过程。近年来, 随着越来越多植物全基因组测序的完成, ABCB亚家族在禾谷类单子叶植物水稻(Oryza sativa)、玉米(Zea mays)和高粱(Sorghum bicolor)中的生物学功能开始有少量报道, 然而多数ABCB转运蛋白的功能尚未得到阐释。该文对拟南芥(Arabidopsis thaliana)和禾谷类作物ABCB转运蛋白的研究进展进行综述, 以期为全面揭示ABCB亚家族生物学功能提供线索。     

The Arabidopsis thaliana ATP-binding cassette proteins: an emerging superfamily

Solute transport systems are one of the major ways in which organisms interact with their environment. Typically, transport is catalysed by integral membrane proteins, of which one of the largest groups is the ATP‐binding cassette (ABC) proteins. On the basis of sequence similarities, a large family of ABC proteins has been identified in Arabidopsis. A total of 60 open reading frames (ORFs) encoding ABC proteins were identified by BLAST homology searching of the nuclear genome. These 60 putative proteins include 89 ABC domains. Based on the assignment of transmembrane domains (TMDs), at least 49 of the 60 proteins identified are ABC transporters. Of these 49 proteins, 28 are full‐length ABC transporters (eight of which have been described previously), and 21 are uncharacterized half‐transporters. Three of the remaining proteins identified appear to be soluble, lacking identifiable TMDs, and most likely have non‐transport functions. The eight other ORFs have homology to the nucleotide‐binding and transmembrane components of multi‐subunit permeases. The majority of ABC proteins found in Arabidopsis can, on the basis of sequence homology, be assigned to subfamilies equivalent to those found in the yeast genome. This assignment of the Arabidopsis ABC proteins into easily recognizable subfamilies (with distinguishable subclusters) is an important first step in the elucidation of their functional role in higher plants.     

The Escherichia coli ATP-binding cassette (ABC) proteins

The recent completion of the Escherichia coli genome sequence ( Blattner et al ., 1997 ) has permitted an analysis of the complement of genomically encoded ATP-binding cassette (ABC) proteins. A total of 79 ABC proteins makes this the largest paralogous family of proteins in E . coli . These 79 proteins include 97 ABC domains (as some proteins include more than one ABC domain) and are components of 69 independent functional systems (as many systems involve more than one ABC domain). The ABC domains are often, but not exclusively, the energy-generating domains of multicomponent membrane-bound transporters. Thus, 57 of the 69 systems are ABC transporters, of which 44 are periplasmic-binding protein-dependent uptake systems and 13 are presumed exporters. The genes encoding these ABC transporters occupy almost 5% of the genome. Of the 12 systems that are not obviously transport related, the function of only one, the excision repair protein UvrA, is known. A phylogenetic analysis suggests that the majority of ABC proteins can be assigned to 10 subfamilies. Together with statistical and, importantly, biological evidence, this analysis provides insight into the evolution and function of the ABC proteins.     

ABC50 interacts with eukaryotic initiation factor 2 and associates with the ribosome in an ATP-dependent manner

Eukaryotic initiation factor 2 (eIF2) plays a key role in the process of translation initiation and in its control. Here we demonstrate that highly purified mammalian eIF2 contains an additional polypeptide of apparent molecular mass of 110 kDa. This polypeptide co-purified with eIF2 through five different chromatography procedures. A cDNA clone encoding the polypeptide was isolated, and its sequence closely matched that of a protein previously termed ABC50, a member of the ATP-binding cassette (ABC) family of proteins. Antibodies to ABC50 co-immunoprecipitated eIF2 and vice versa, indicating that the two proteins interact. The presence of ABC50 had no effect upon the ability of eIF2 to bind GDP but markedly enhanced the association of methionyl-tRNA with the factor. Unlike the majority of ABC proteins, which are membrane-associated transporters, ABC50 associates with the ribosome and co-sediments in sucrose gradients with the 40 and 60 S ribosomal subunits. The association of ABC50 with ribosomal subunits was increased by ATP and decreased by ADP. ABC50 is related to GCN20 and eEF3, two yeast ABC proteins that are not membrane-associated transporters and are instead implicated in mRNA translation and/or its control. Thus, these data identify ABC50 as a third ABC protein with a likely function in mRNA translation, which associates with eIF2 and with ribosomes.     

The ABC transporters of Saccharomyces cerevisiae

The ABC transporters (ATP Binding Cassette) compose one of the bigest protein family with the great medical, industrial and economical impact. They are found in all organism from bacteria to man. ABC proteins are responsible for resistance of microorganism to antibiotics and fungicides and multidrug resistance of cancer cells. Mutations in ABC transporters genes cause seriuos deseases like cystic fibrosis, adrenoleucodystrophy or ataxia. Transport catalized by ABC proteins is charged with energy from the ATP hydrolysis. The ABC superfamily contains transporters, canals, receptors. Analysis of the Saccharomyces cerevisiae genome allowed to distinguish 30 potential ABC proteins which are classified into 6 subfamilies. The structural and functional similarity of the yeast and human ABC proteins allowes to use the S. cerevisiae as a model organism for ABC transporters characterisation. In this work the present state of knowleadge on yeast S. cerevisiae ABC proteins was summarised.     

The N-terminal region of ABC50 interacts with eukaryotic initiation factor eIF2 and is a target for regulatory phosphorylation by CK2

ABC50 is an ABC (ATP-binding cassette) protein which, unlike most ABC proteins, lacks membrane-spanning domains. ABC50 interacts with eIF2 (eukaryotic initiation factor 2), a protein that plays a key role in translation initiation and in its control, and in regulation of ribosomes. Here, we establish that the interaction of ABC50 with eIF2 involves features in the N-terminal domain of ABC50, the region of ABC50 that differs most markedly from other ABC proteins. This region also shows no apparent similarity to the eIF2-binding domains of other partners of eIF2. In contrast, the N-terminus of ABC50 cannot bind to ribosomes by itself, but it can in conjunction with one of the nucleotide-binding domains. We demonstrate that ABC50 is a phosphoprotein and is phosphorylated at two sites by CK2. These sites, Ser-109 and Ser-140, lie in the N-terminal part of ABC50 but are not required for the binding of ABC50 to eIF2. Expression of a mutant of ABC50 in which both sites are mutated to alanine markedly decreased the association of eIF2 with 80S ribosomal and polysomal fractions.     

One of the major sulphated proteins secreted by rat hepatocytes contains low-sulphated chondroitin sulphate.

When isolated hepatocytes are incubated with 35SO4(2-), a specific set of secretory proteins is labelled. One of these proteins is electrophoretically heterogeneous, with an apparent molecular mass of 35-45 kDa [Marcks von Würtemberg & Fries (1989) Biochemistry 28, 4088-4093]. Here we report that treatment with chondroitinase ABC converted the broad electrophoretic band of this protein, with a 50-60% loss of radioactivity, into a relatively homogeneous band with a molecular mass of 28 kDa. Size determination by gel chromatography of the protein's oligosaccharide chain (released by alkali treatment) indicated that it contained about 40 hexose units. Similar analysis of the enzyme-resistant oligosaccharide chain remaining linked to the protein after chondroitinase ABC treatment indicated a size of between six and eight hexose units. These observations suggest that the protein's oligosaccharide chain carries only three or four sulphate groups, of which one or two are located close to the polypeptide chain. Consistent with this hypothesis, the free oligosaccharide behaved like a low-sulphated glycosaminoglycan upon ion-exchange chromatography.     

Cystic fibrosis transmembrane conductance regulator (CFTR): Making an ion channel out of an active transporter structure

Cystic fibrosis is caused by mutations in the cystic fibrosis transmembrane conductance regulator (CFTR). CFTR is a member of the ATP-binding cassette (ABC) family of membrane transport proteins, most members of which function as ATP-dependent pumps. CFTR is unique among human ABC proteins in functioning not as a pump, but as an ion channel. Recent structural data has indicated that CFTR shares broadly similar overall architecture and ATP-dependent conformational changes as other ABC proteins. Functional investigations suggest that CFTR has a unique open portal connecting the cytoplasm to the transmembrane channel pore, that allows for a continuous pathway for Cl^? ions to cross the membrane in one conformation. This lateral portal may be what allows CFTR to function as an ion channel rather than as a pump, suggesting a plausible mechanism by which channel function may have evolved in CFTR.     

X-Linked Adrenoleukodystrophy: Genes,Mutations, and Phenotypes

X-linked adrenoleukodystrophy (X-ALD) is a complex and perplexing neurodegenerative disorder. The metabolic abnormality, elevated levels of very long-chain fatty acids in tissues and plasma, and the biochemical defect, reduced peroxisomal very long-chain acyl-CoA synthetase (VLCS) activity, are ubiquitous features of the disease. However, clinical manifestations are highly variable with regard to time of onset, site of initial pathology and rate of progression. In addition, the abnormal gene in X-ALD is not the gene for VLCS. Rather, it encodes a peroxisomal membrane protein with homology to the ATP-binding cassette (ABC) transmembrane transporter superfamily of proteins. The X-ALD protein (ALDP) is closely related to three other peroxisomal membrane ABC proteins. In this report we summarize all known X-ALD mutations and establish the lack of an X-ALD genotype/phenotype correlation. We compare the evolutionary relationships among peroxisomal ABC proteins, demonstrate that ALDP forms homodimers with itself and heterodimers with other peroxisomal ABC proteins and present cDNA complementation studies suggesting that the peroxisomal ABC proteins have overlapping functions. We also establish that there are at least two peroxisomal VLCS activities, one that is ALDP dependent and one that is ALDP independent. Finally, we discuss variable expression of the peroxisomal ABC proteins and ALDP independent VLCS in relation to the variable clinical presentations of X-ALD.