大蒜、绊根草中重金属抗性分子机制的研究

日益加剧的重金属污染已经危害到了全球的生态环境以及人类健康。在分子水平上阐明植物中的重金属抗性机制并应用于环境修复和绿色农业是植物科学和环境科学以及农业科学的交叉点和新的生长点。为了了解植物重金属抗性的分子机制，我们的研究主要是从重金属抗性植物材料大蒜(Allium sativumL．)和绊根草(Cynodon dactylon)中分离重金属抗性相关基因，并研究它们在重金属抗性机制中的功能。 在高等植物中有迹象表明，一种富含半胱氨酸的低分子量蛋白．类金属硫蛋白 (Metallothioneins Like，MTs Like)和一类具有Y-(Glu-Cys) n-Gly特殊结构的多肽一植物络合素(Phytochelatins，PCs)在重金属抗性机制中占有重要地位。然而人们对于同一种植物中这两种重金属结合肽作用的相互关系还缺乏了解，同时对于MT Like基因以及PCs合酶基因在同一种植物中的表达模式如金属离子专一性、时空表达特点等，还投有文献报道，因此本文将首先以这两个基因为切入点进行研究。 本研究采用RACE的方法，从大蒜中分离得到了类金属硫蛋白(MT-Like)的cDNA序列(GenBank Accession No.AY050510)，PCR和SoutheLrn Blot分析表明，大蒜基因组中不仅存在类金属硫蛋白基因，而且可能以基因家族的形式存在。对获得的MT Like cDNA进行的序列分析及同源性分析表明，大蒜MT Like cDNA含有一个完整的开放阅读框架，编码73个氨基酸，其中12个为半胱氨酸，占氨基酸总数的1 6.4%，并与其他植物如水稻、小麦、紫羊茅草中的类金属硫蛋白基因同源性较高，其中最高达89%。对该基因编码的氨基酸序列和结构分析表明在N-端、c-端结构域中分别含有3个典型的金属硫蛋白的结构模式Cys-Xaa-Cys，属于典型的Type-1类金属硫蛋白。这些Cys-Xaa-Cys特征结构表明大蒜MT Like基因编码的蛋白可以结合二价金属离子。重金属胁迫下大蒜根中MT Like基因在转录水平的表达检测表明，MT Like基因的表达受重金属离子Cu2+、Cd2+的诱导，暗示MT Like基因在大蒜对重金属的抗性中有重要作用。此外，用能谱电镜技术研究大蒜中重金属的积累与分布，以及用组织原位杂交技术分析MT Like基因的表达定位与重金属的积累、转运的关系已在进行之中。 植物络合素也是富含巯基的多肽化合物，在重金属抗性中起重要作用。由植物络合素结构中存在的Y一酰胺键或β-Ala可知PCs不是基因表达的直接产物，而是以GSH为前体的酶促反应产物。目前已知y一谷氨酰半胱氨酸二肽转肽酶(简称为PCs合酶，phytochelatin synthase，PCS)是PCs合成途径的关键酶，编码这一关键酶的基因目前已在小麦、拟南芥菜和裂殖酵母中克隆。由于这一基因在不同物种中的保守性较低，其克隆较困难。本研究通过设计植物络合素台酶基因简并引物，从大蒜中扩增得到了345bp的cDNA序列。序列分析和推测的氨基酸序列同源性比较表明，此序列的翻译产物与已知的植物络合素合酶同源性最高，此cDNA序列应为大蒜植物络合素合酶基因的部分cDNA序列(GenBank Accession No.AF384110)。目前大蒜植物络台素合酶基因的全长序列的扩增，以及这两种与重金属抗性有关的基因(MT Like，PCS)的表达模式仍在研究中。 本文还尝试了利用酵母重金属敏感突变株M379/8功能互补的方法从重金属抗性植物绊根革中分离新的重金属抗性相关基因。构建了用于转化的酵母质粒表达文库，探索了酵母转化体系建立的条件。曾尝试多种转化方法，并对其中的条件进行了优化改进。下一步的工作将集中在合适的酵母突变体的筛选或穿梭表达载体的选择标记基因替换上

绊根草重金属抗性相关基因的克隆及其功能分析及可耐受偏二甲肼的芦苇变异株系的筛选

本研究利用酵母功能互补方法和RACE的方法从具有较强抗逆能力的绊根草中克隆了9个与重金属抗性相关的克隆，并对部分基因的表达调控及功能进行了初步研究。同时还利用细胞工程技术筛选到了具有较强的耐受火箭推进齐-偏二甲肼(UDMH)的芦苇的变异株系，为以后用人工湿地系统处理受偏二甲肼污染的废水奠定了基础。 本研究通过酵母功能互补法克隆到了五个基因，分别为CdSRP、CdTETH、 CdASP、CdMT2和CdTER1。CdSRP可能是一种衰老相关基因;CdTETH编码的产物可能是组成TRAPP复合体的一个亚基;CdASP是一个功能未知的基因;CdMT2是一个编码Type Ⅱ型金属硫蛋白基因;CdTER1可能是编码一个TERl-like家族蛋白成员的基因。用这五个基因分别转化因Acr基因缺失而对As敏感的酵母菌株FD236-6A，所获得的转化子对As的抗性均有提高，其中以CdMT2、CdTER1和CdASP的作用最为明显。这些基因的表达调控方式以及与其它重金属抗性的关系正在研究中。 本研究还利用RACE的方法克隆了一个谷胱甘肽S-转移酶基因，CdGSTFl;两个植物络合素合酶基因，CdPCSI和CdPCSⅡ，和一个TypeⅠ型金属硫蛋白基因CdMT1。CdGSTF1属于phi类GST基因，Northern-blotting分析表明，CdGSTF1在绊根草根部的表达受Cd2+的诱导，暗示其可能具有解除氧自由基或氢过氧化物的毒性的作用。CdPCSI和CdPCSⅡ的同源性较高，表明绊根草含有两个以上的PCs合酶的基因。参照前人的方法对CdPCSI和CdPCSII的氨基酸序列进行分析，发现它们含有六个非常相近的Cd2+结合位点，这两个基因的功能及其调控方式有何差异尚需进一步的研究。cdMT1与用酵母功能互补法克隆到的CdMT2属于不同类型的MT基因，对它们之间很可能存在的功能、组织特异性等方面的差异性进行了讨论。 四氧化二氮／偏二甲肼是常用的航天器双组元液体推进剂。偏二甲肼易挥发，有致癌、致畸、致突变的毒性。在推进剂贮存、运输、转注、火箭发动机试车、火箭发射、管道及设备冲洗中产生的含有偏二甲肼的废水能够对卫星发射基地的地下水源和空气造成污染。因此迫切需要培育能够净化偏二甲肼污水的植物。 本研究利用生长在卫星发射基地的野生芦苇的种子诱导愈伤组织，进而通过逐步提高偏二甲肼筛选压力的方式从中筛选出具有较强抗性的愈伤组织，然后诱导其分化。目前已经得到能够在含有1.63 mmol/L和3.26 mmol/L偏二甲肼的分化培养基中生长良好的芦苇再生苗，并已成功转移至温室中。抗性分化苗对污水的处理效果和耐受偏二甲肼的机理正在研究中。

大车前（Plantago major L. "Giant Turkish."）体外优化再生体系的建立及Na+/H+逆向转运蛋白基因SeNHX1 和TtNHX1 的功能鉴定

大车前（Plantago major L. "Giant Turkish."）不仅有很高的药用价值，在生态学研究方面也是重要模式植物。大车前的组织培养工作，目前报道很少。对其组织培养体系的建立，为筛选大车前耐盐突变体和基因转化建立高效的体外再生系统和实验平台体系。通过愈伤组织诱导和直接不定芽再生途径， 建立了大车前（Plantago major L. "Giant Turkish."）的快速高效再生系统。叶片外植体在含有1.0 mg/L NAA的MS培养基中培养3周后，形成愈伤组织，愈伤组织在含4.0 mg/L 6-BA的MS培养基中成功再生，得到完整植株。种子外植体在含0.2 mg/L IAA和1.0 mg/L TDZ的MS培养基中培养4周后产生大量的丛生芽，对9株再生植株进行RAPD检测表明，部分植株在DNA水平上发生了变异。 植物抵御盐胁迫的一个重要机制是在液泡中积累Na+，从而使细胞质内Na+保持在较低水平，并且降低细胞渗透势。Na+运输到液泡是由液泡Na+/H+逆向转运蛋白完成的。本实验室已从盐生植物盐角草（Salicornia europaea）和番杏（Tetragonia tetragonioides）中分别克隆得到SeNHX1和TtNHX1基因。本文研究了SeNHX1和TtNHX1基因在酵母突变体里的作用。TtNHX1和SeNHX1蛋白在缺陷型酵母菌株里的表达能够提高这些菌株对NaCl、LiCl和潮霉素的抗性，提高到与野生型相当的抗性水平。说明TtNHX1和SeNHX1有着与酵母ScNHX1相似的细胞定位和作用机制，是ScNHX1的功能类似蛋白。

DnaJ-like protein gene sll1384 is involved in phototaxis in Synechocystis sp PCC 6803

In Synechocystis sp. PCC 6803, gene sll1384 encodes a protein with a DnaJ domain at its N-terminal portion and a TPR domain at the C-terminal portion. An sll1384 mutant shows no difference from the wild type in adaptation to different temperatures, but almost completely loses its capability of phototactic movement. After complementation with sll1384, the mutant regains the phototaxis. As shown with electron microscopy, on the cell surface, mutant cells have pili that appear to be the same as that of the wild type. Also, the transformation efficiency remains unchanged in the mutant. It is postulated that Sll1384 regulates phototaxis of Synechocystis through protein-protein interaction. It is the first DnaJ-like protein gene identified in a cyanobacterium for a role in phototaxis.

Identification of a gene, ccr-1 (sll1242), required for chill-light tolerance and growth at 15 degrees C in Synechocystis sp PCC 6803

Synechocystis sp. PCC 6803 exposed to chill (5 degrees C)-light (100 mu mol photons m(-2) s(-1)) stress loses its ability to reinitiate growth. From a random insertion mutant library of Synechocystis sp. PCC 6803, a sll1242 mutant showing increased sensitivity to chill plus light was isolated. Mutant reconstruction and complementation with the wild-type gene confirmed the role of sll1242 in maintaining chill-light tolerance. At 15 degrees C, the autotrophic and mixotrophic growth of the mutant were both inhibited, paralleled by decreased photosynthetic activity. The expression of sll1242 was upregulated in Synechocystis sp. PCC 6803 after transfer from 30 to 15 degrees C at a photosynthetic photon flux density of 30 mu mol photons m(-2) S-1. sll1242, named ccr (cyanobacterial cold resistance gene)- 1, may be required for cold acclimation of cyanobacteria in light.

alr0117, a two-component histidine kinase gene, is involved in heterocyst development in Anabaena sp PCC 7120

Anabaena sp. PCC; 7120 was mutagenized by transposon Tn5-1087b, generating a mutant whose heterocysts lack the envelope polysaccharide layer. The transposon was located between nucleotides 342 and 343 of alr0117, a 918 bp gene encoding a histidine kinase for a two-component regulatory system. Complementation of the mutant with a DNA fragment containing alr0117 and targeted inactivation of the gene confirmed that alr0117 is involved in heterocyst development. RT-PCR showed that alr0117 was constitutively expressed in the presence or absence of a combined-nitrogen source. hepA and patB, the two genes turned on during wild-type heterocyst development, were no longer activated in an alr0117-null mutant. The two-component signal transduction system involving alr0117 may control the formation of the envelope polysaccharide layer and certain late events essential to the function of heterocysts.

Investigation of EscA as a chaperone for the Edwardsiella tarda type III secretion system putative translocon component EseC

Edwardsiella tarda is an important Gram-negative enteric pathogen affecting both animals and humans. It possesses a type III secretion system (T3SS) essential for pathogenesis. EseB, EseC and EseD have been shown to form a translocon complex after secretion, while EscC functions as a T3SS chaperone for EseB and EseD. In this paper we identify EscA, a protein required for accumulation and proper secretion of another translocon component, EseC. The escA gene is located upstream of eseC and the EscA protein has the characteristics of T3SS chaperones. Cell fractionation experiments indicated that EscA is located in the cytoplasm and on the cytoplasmic membrane. Mutation with in-frame deletion of escA greatly decreased the secretion of EseC, while complementation of escA restored the wild-type secretion phenotype. The stabilization and accumulation of EseC in the cytoplasm were also affected in the absence of EscA. Mutation of escA did not affect the transcription of eseC but reduced the accumulation level of EseC as measured by using an EseC-LacZ fusion protein in Ed. tarda. Co-purification and co-immunoprecipitation studies demonstrated a specific interaction between EscA and EseC. Further analysis showed that residues 31-137 of EseC are required for EseC-EscA interaction, Mutation of EseC residues 31-137 reduced the secretion and accumulation of EseC in Ed. tarda. Finally, infection experiments showed that mutations of EscA and residues 31-137 of EseC increased the LD50 by approximately 10-fold in blue gourami fish. These results indicated that EscA functions as a specific chaperone for EseC and contributes to the virulence of Ed. tarda.

Using the ribosomal internal transcribed spacer (ITS) as a complement marker for species identification of red macroalgae

Barcodes based on mitochondrial cytochrome oxidase (mtDNA CO1) sequences are being used for broad taxonomic groups of animals with demonstrated success in species identification and cryptic species discovery, but it has become clear that complementation by a nuclear marker system is necessary, in particular for the barcoding of plants. Here, we propose the nuclear internal transcribed spacer (ITS) as a potentially usable and complementary marker for species identification of red macroalgae, as well as present a primary workflow for species barcoding. Data show that for most red macroalgal genera (except members of the family Delesseriaceae), the size of ITS region ranges from 600 to 1200 bp, and contains enough variation to generate unique identifiers at either the species or genus levels. Consistent with previous studies, we found that the ITS sequence can resolve closely related species with the same fidelity as mtDNA CO1. Significantly, we confirmed that length polymorphism in the ITS region (including 5.8S rRNA gene) can be utilized as a character to discriminate red macroalgal species. As a complementary marker, the verifiable nuclear ITS region can speed routine identification and the detection of species, advance ecological and taxonomic inquiry, and permit rapid and accurate analysis of red macroalgae.

EscC is a chaperone for the Edwardsiella tarda type III secretion system putative translocon components EseB and EseD

Edwardsiella tarda is a Gram-negative enteric pathogen that causes disease in both humans and animals. Recently, a type III secretion system (T3SS) has been found to contribute to Ed. tarda pathogenesis. EseB, EseC and EseD were shown to be secreted by the T3SS and to be the major components of the extracellular proteins (ECPs). Based on sequence similarity, they have been proposed to function as the 'translocon' of the T3SS needle structure. In this study, it was shown that EseB, EseC and EseD formed a protein complex after secretion, which is consistent with their possible roles as translocon components. The secretion of EseB and EseD was dependent on EscC (previously named Orf2). EscC has the characteristics of a chaperone; it is a small protein (13 kDa), located next to the translocators in the T3SS gene cluster, and has a coiled-coil structure at the N-terminal region as predicted by COILS. An in-frame deletion of escC abolished the secretion of EseB and EseD, and complementation of Delta escC restored the export of EseB and EseD into the culture supernatant. Further studies showed that EscC is not a secreted protein and is located on the membrane and in the cytoplasm. Mutation of escC did not affect the transcription of eseB but reduced the amount of EseB as measured by using an EseB-LacZ fusion protein in Ed. tarda. Co-purification studies demonstrated that EscC formed complexes with EseB and EseD. The results suggest that EscC functions as a T3SS chaperone for the putative translocon components EseB and EseD in Ed. tarda.