水稻磷酸盐转运蛋白基因的克隆、表达及功能分析

以水稻叶片为材料, 设计一对特异引物, 获得了编码磷酸盐转运蛋白基因OsPT6:1. 聚类和氨基酸保守位点分析指出该基因可能为水稻高亲和力磷酸盐转运蛋白编码基因. 原位杂交与RT-PCR表达结果确定此基因在根与叶片中均表达, 尤以低磷诱导下叶片的叶肉细胞表达量最高. 同源重组表明该基因的表达可以提高毕氏酵母对磷素的吸收效率, 同时其基因的导入可以使高亲和力磷酸盐转运蛋白缺失的酵母突变体的磷素吸收功能得以恢复. 以上结果表明, OsPT6:1为水稻高亲和力磷酸盐转运蛋白的编码基因.     

植物菌根共生磷酸盐转运蛋白

大多数植物能和丛枝菌根（arbuscular mycorrhiza, AM）真菌形成菌根共生体。AM能够促进植物对土壤中矿质营养的吸收,尤其是磷的吸收。磷的吸收和转运由磷酸盐转运蛋白介导。总结了植物AM磷酸盐转运蛋白及其结构特征,分析其分类及系统进化,并综述了AM磷酸盐转运蛋白介导的磷的吸收和转运过程及其基因的表达调控。植物AM磷酸盐转运蛋白属于Pht1家族成员,它不仅对磷的吸收和转运是必需的,而且对AM共生也至关重要,为进一步了解菌根形成的分子机理及信号转导途径提供了理论基础。     

米曲霉异源蛋白表达系统研究进展及展望

米曲霉作为一种重要的工业微生物,在异源蛋白表达方面已有广泛应用,受限于被表达蛋白的修饰及分泌过程,目前实际生产使用的基因供体主要局限于其他真菌,尤其是丝状真菌。当外源基因来源于植物、昆虫和哺乳动物时,米曲霉所生产的异源蛋白产量及生物活性往往不尽如人意。本文综述了米曲霉作为宿主表达异源蛋白的研究进展,包括其现有的遗传操作手段及异源表达方面的应用及探索,重点介绍了应用过程中面临的挑战和解决策略,另外,对米曲霉表达异源蛋白的应用前景及发展方向进行了展望。     

茶树硝酸盐转运蛋白基因的克隆和表达分析

硝酸盐转运蛋白（NRT）是植物吸收和利用硝态氮的一种关键蛋白。运用RACE技术从茶树中扩增出NRT基因的cDNA,并利用实时荧光定量PCR检测了CsNRT基因在不同茶树器官与品种之间的差异表达。结果表明：CsNRT基因的cDNA全长2 061 bp,开放阅读框为1 818 bp,编码含由605个氨基酸组成的蛋白质,GenBank登录号为KJ160503,属于NRT2基因家族。CsNRT为组成型基因,对不同处理的水培茶苗进行定量表达分析显示,该基因在根、茎、叶中都有表达,其中在根部的表达水平最高,1.0 mmol·L-1的NO3-可诱导其表达量上升7.53倍。不同茶树品种中CsNRT基因的表达也有较大差异,‘龙井长叶’和‘凫早2号’的表达量较高,前者强烈响应0.5和1.0 mmol·L-1 NO3-的诱导,后者的响应浓度为1.0和2.0mmol·L-1,而‘舒茶早’在各浓度下的表达差异不明显。     

丝状真菌异源蛋白表达系统研究进展

丝状真菌,俗称霉菌,在食品工业中被用于生产多种生物酶和有机酸。近年来,人们发现丝状真菌具有分泌量大、表达的蛋白有天然活性等特点,非常适合作为同源和异源重组蛋白的表达宿主,因此被广泛研究和探讨。简要综述了以黑曲霉为代表的几种常被用作蛋白表达宿主的丝状真菌的特点、应用中的主要问题和基本解决方案,以及近年关于丝状真菌表达系统的最佳培养条件和发酵条件的研究进展。     

丝状真菌高效表达异源蛋白研究进展

丝状真菌是具有高效分泌蛋白质潜力的真核表达系统, 能对蛋白质进行翻译后修饰, 如蛋白质糖基化等; 并且比植物、昆虫和哺乳动物细胞具有更快的生长速率。近年来, 随着真菌分子遗传技术和菌种改良策略的进步, 尤其是真菌基因组学的发展, 利用丝状真菌生产异源蛋白越来越受到关注。综述了丝状真菌作为细胞工厂生产异源蛋白的最新探索与进展, 其中包括功能基因组学在蛋白表达与分泌研究中的应用, 同时探讨了异源蛋白表达和生产的改进策略。     

丝状真菌高效表达异源蛋白研究进展

丝状真菌是具有高效分泌蛋白质潜力的真核表达系统, 能对蛋白质进行翻译后修饰, 如蛋白质糖基化等; 并且比植物、昆虫和哺乳动物细胞具有更快的生长速率。近年来, 随着真菌分子遗传技术和菌种改良策略的进步, 尤其是真菌基因组学的发展, 利用丝状真菌生产异源蛋白越来越受到关注。综述了丝状真菌作为细胞工厂生产异源蛋白的最新探索与进展, 其中包括功能基因组学在蛋白表达与分泌研究中的应用, 同时探讨了异源蛋白表达和生产的改进策略。     

金龟子绿僵菌羧基转运蛋白基因MaJEN1及其启动子的克隆与分析

用YADE法扩增了球孢白僵菌T—DNA插入突变体T12中与T—DNA左边界相连的基因组序列。在此基础上得到了金龟子绿僵菌的羧基转运蛋白的全长cDNA,MaJEN1。MaJEN1全长1695bp,其中含有长为1524bp的开放阅读框(0RF),编码508个氨基酸的蛋白。氨基酸序列与粗糙脉孢霉和啤酒酵母菌的羧基转运蛋白JEN1相似性分别为69％和31％。采用PCR扩增得到了MaJEN1的基因组序列GMaJEN1,序列分析发现,GMaJEN1含有两个内含子。Southern杂交发现GMaJEN1在金龟子绿僵菌基因组上为单拷贝。利用RT—PCR法对MaJEN1的表达特性进行了分析,结果表明MaJEN1在蟑螂壳诱导培养基中表达,在该培养基中的表达受葡糖糖抑制。进一步采用YADE法得到了长为1626bp的GMaJEN1上游序列,其中含有可能的葡萄糖抑制调控序列。     

积磷小月菌调控蛋白Mlp21700的异源表达及其与多聚磷酸盐(Poly-P)代谢基因启动子的结合

【背景】积磷小月菌(Microlunatus phosphovorus)是重要的聚磷微生物,在好氧条件下积累聚磷酸盐并在厌氧条件分解聚磷酸盐,这个过程可能受到精细的基因调控。【目的】利用凝胶迁移实验(EMSA)分析调控蛋白Mlp21700结合的多聚磷酸盐(Poly-P)代谢基因启动子,找到Mlp21700可能的调控靶点。【方法】以积磷小月菌JN459菌株的基因组DNA为模板,PCR扩增Mlp21700编码序列,构建重组质粒p ET28a-21700并转化到大肠杆菌Transetta(DE3)菌株,诱导表达后采用非变性方法纯化获得Mlp21700融合蛋白。利用PCR方法分别扩增各个Poly-P代谢基因的启动子,用生物素标记后作为探针。采用EMSA分析Mlp21700在试验条件下是否结合启动子以及结合强度。【结果】DNA测序和酶切验证表明p ET28a-21700携带正确的Mlp21700编码序列。SDS-PAGE分析显示试验条件下Transetta(DE3)菌株大量表达可溶性Mlp21700,纯化的重组Mlp21700蛋白纯度大于90%,含量为0.64 mg/mL。EMSA分析表明在试验条件下Mlp21700能够结合Mlp26610基因ppgk和Mlp44770基因ppx的启动子。【结论】调控蛋白Mlp21700可能参与Mlp26610和Mlp44770基因的转录调控,进而调控Poly-P的分解过程。     

陆地棉蔗糖转运蛋白基因家族的鉴定及表达分析

蔗糖转运蛋白(SUT)在蔗糖从“源”到“库”的运输与分配过程中发挥着重要作用。该研究基于最新公布的陆地棉基因组数据,利用生物信息学和荧光定量PCR等方法,对陆地棉SUT基因家族进行全基因组鉴定,并对他们的表达特性进行系统分析。结果显示：(1)在陆地棉基因组中,共鉴定到18个GhSUT基因(GhSUT1 GhSUT18),他们不均匀地分布在陆地棉11条染色体上。(2)GhSUT蛋白间序列一致性很高,均具有11～12个跨膜结构域,且都定位于质膜。(3)进化关系分析表明,陆地棉GhSUT蛋白主要分布在双子叶植物特有的SUT1亚组,以及单、双子叶植物共有的SUT2亚组和SUT4亚组,其中SUT1亚组成员最多,包含8个GhSUT基因。(4)位于同一亚组的GhSUT基因具有相似的内含子 外显子分布模式,不同亚组间GhSUT基因内含子/外显子数目差异很大。(5)转录组分析表明,GhSUT基因在表达水平上存在差异,GhSUT1和GhSUT10在被检测的组织不表达,GhSUT5、GhSUT14、GhSUT7和GhSUT16在被检测的组织表达量较低,其他GhSUT基因在被检测的组织具有较高的表达水平;另外,GhSUT基因的表达具有组织特异性,其中GhSUT2和GhSUT11主要在“源”和“库”器官中表达,GhSUT6和GhSUT15主要在“库”器官中表达,而GhSUT9和GhSUT18主要在纤维中表达。(6)荧光定量PCR分析表明,GhSUT2在“源”和“库”器官中均具有较高的表达水平,GhSUT6主要在“库”器官包括根、花瓣、纤维和茎中表达,在“源”器官(叶片)中表达量很低;GhSUT18主要在纤维中特异性高表达,在其他组织表达量很低。研究表明,实验验证结果与转录组分析结果相对一致。该研究结果为进一步研究SUT家族基因的功能提供了重要的基因信息,并为棉花产量的提高和纤维品质的改良奠定了理论依据。     

Isolation and characterization of a sodium-dependent phosphate transporter gene in Dunaliella viridis

A sodium-dependent phosphate transporter gene, DvSPT1, was isolated from a cDNA library using a probe derived from a subtracted cDNA library of Dunaliella viridis. Sequencing analyses revealed a cDNA sequence of 2649 bp long and encoded an open-reading frame consisting of 672 amino acids. The deduced amino acid sequence of DvSPT1 exhibited 31.2% identity to that of TcPHO from Tetraselmis chui. Hydrophobicity and secondary structure prediction revealed 11 conserved transmembrane domains similar to those found in PHO89 from Saccharomyces cerevisiae and PHO4 from Neurospora crassa. Northern blot analysis indicated that the DvSPT1 expression was induced upon NaCl hyperosmotic stress or phosphate depletion. Functional characterization in yeast Na+ export pump mutant G19 suggested that DvSPT1 encoded a Na+ transporter protein. The gene sequence of GDvSPT1 (7922 bp) was isolated from a genomic library of D. viridis. Southern blot analysis indicated that there exist at least two homologous genes in D. viridis.     

外源基因在大肠杆菌中的高效表达

为了提高外源蛋白在大杨杆菌中的表达量,人们对大肠杆菌表达系统进行了许多研究。作者综述了有关外源基因在大肠杆菌中高效表达的研究进展。     

Isolation and characterization of root-specific phosphate transporter promoters from Medicago trunatula

Promoters of phosphate transporter genes MtPT1 and MtPT2 of Medicago truncatula were isolated by utilizing the gene-space sequence information and by screening of a genomic library, respectively. Two reporter genes, beta-glucuronidase (GUS) and green fluorescent protein (GFP) were placed under the control of the MtPT1 and MtPT2 promoters. These chimeric transgenes were introduced into Arabidopsis thaliana and transgenic roots of M. truncatula, and expression patterns of the reporter genes were assayed in plants grown under different phosphate (Pi) concentrations. The expression of GUS and GFP was only observed in root tissues, and the levels of expression decreased with increasing concentrations of Pi. GUS activities in roots of transgenic plants decreased 10-fold when the plants were transferred from 10 microM to 2 mM Pi conditions, however, when the plants were transferred back to 10 microM Pi conditions, GUS expression reversed back to the original level. The two promoters lead to different expression patterns inside root tissues. The MtPT1 promoter leads to preferential expression in root epidermal and cortex cells, while MtPT2 promoter results in strong expression in the vascular cylinder in the center of roots. Promoter deletion analyses revealed possible sequences involved in root specificity and Pi responsiveness. The promoters are valuable tools for defined engineering of plants, particularly for root-specific expression of transgenes.     

桦褐孔菌膜二肽酶在巴斯德毕赤酵母中的分泌表达

本研究利用巴斯德毕赤酵母Pichia pastoris蛋白表达体系表达了药用担子菌桦褐孔菌的一个二肽酶基因。该二肽酶基因编码区全长1814bp,包含6个内含子,编码465个氨基酸。生物信息学分析发现,二肽酶基因编码的蛋白中不含信号肽序列,但在第55–77位氨基酸之间存在一个跨膜结构。将含跨膜结构和去跨膜结构蛋白的cDNA序列分别克隆到酵母分泌型表达载体pPICZαA上,电转化至巴斯德毕赤酵母X-33中,用1%(V/V)甲醇诱导重组菌株表达目标蛋白,采用SDS-PAGE和Western-blot检测表达蛋白。结果显示,巴斯德毕赤酵母可表达含跨膜结构的完整基因,但目标蛋白不能分泌到胞外,存在于破碎细胞的沉淀中,且没有催化活性;而去跨膜结构的蛋白则可分泌表达到胞外,并具有催化活性。Ni-NTA纯化去跨膜结构的桦褐孔菌二肽酶浓度可达0.12mg/mL,并发现其在pH 7.3、反应温度50℃、反应时间2h的条件下,以Gly-Gly为底物时,其比活为433U/mg。同时检测到其对Ile-Leu、Trp-Trp和Phe-Phe具有较高的水解活性。     

Molecular cloning and functional analysis of a H+-dependent phosphate transporter gene from the ectomycorrhizal fungus Boletus edulis in southwest China

Phosphate transporters (PTs), as entry points for phosphorus (P) in organisms, are involved in a number of P nutrition processes such as phosphate uptake, transport, and transfer. In the study, a PT gene 1632 bp long (named BePT) was cloned, identified, and functionally characterized from Boletus edulis. BePT was expected to encode a polypeptide with 543 amino acid residues. The BePT polypeptide belonged to the major facilitator superfamily and showed a high degree of sequence identity to the Pht1 family. A topology model revealed that BePT exhibited 12 transmembrane helices, divided into two halves, and connected by a large hydrophilic loop in the middle. A yeast mutant complementation analysis suggested that BePT was a functional PT which mediated orthophosphate uptake of yeast at micromolar concentrations. Green fluorescent protein–BePT fusion proteins expressed were extensively restricted to the plasma membrane in BePT transformed yeast, and its activity was dependent on electrochemical membrane potential. In vitro, quantitative PCR confirmed that the expression of BePT was significantly upregulated at lower phosphorus availability, which may enhance phosphate uptake and transport under phosphate starvation. Our results suggest that BePT plays a key role in phosphate acquisition in the ectomycorrhizal fungus B. edulis.     

Cloning, expression and function of phosphate transporter encoded gene in Oryza sativa L.

OsPT6:1, a phosphate transporter encoding gene from the leaf samples of Oryza sativa, was identified through PCR with specifically designed primers. The phylogenetic analysis and the conserved amino acid residue site detection suggested OsPT6:1 a possible high-affinity phosphate transporter encoding gene. In situ hybridization and RT-PCR demonstrated the expression of OsPT6:1 in both roots and leaves. The peak expression signal was observed in mesophyll cells under low phosphorus (P) induction. A homologous recombination study indicated that OsPT6:1 can enhance the Pi uptake efficiency of Pichia pastoris. At the meantime, the introduction of OsPT6:1 was able to complement the Pi uptake function of yeast cells with high-affinity phosphate transporters deficient. Those results substantiated our contention that OsPT6:1 encoded a high-affinity phosphate transporter of Oryza sativa. These authors contributed equally to this work.     

Cloning,expression and function of phosphate transporter encoded gene in Oryza sativa L.

OsPT6:1,a phosphate transporter encoding gene from the leaf samples of Oryza sativa, was identified through PCR with specifically designed primers.The phylogenetic analysis and the conserved amino acid residue site detection suggested OsPT6:1 a possible high-affinity phosphate transporter encoding gene.In situ hybridization and RT-PCR demonstrated the expression of OsPT6:1 in both roots and leaves.The peak expression signal was observed in mesophyll cells under low phosphorus(P)induction.A homologous recombination study indicated that OsPT6:1 can enhance the Pi uptake efficiency of Pichia pastoris.At the meantime,the introduction of OsPT6:1 was able to complement the Pi uptake function of yeast cells with high-affinity phosphate transporters de- ficient.Those results substantiated our contention that OsPT6:1 encoded a high-affinity phosphate transporter of Oryza sativa.