基于荧光激活细胞分选技术的超高通量酶活性筛选方法及其应用

基于荧光激活细胞分选(FACS)技术的超高通量酶活性筛选方法是新出现的一类高通量筛选技术.它利用流式细胞仪高灵敏度、高通量的特点,能以极高的速度(108/天)对大容量酶基因文库进行筛选.FACS筛选技术的出现突破了常规筛选方法低效、耗时、费力等瓶颈问题,极大地提升了人类对大容量基因文库的探索能力,因此在新酶基因筛选、酶活性检测、酶定向进化等领域有广泛的应用潜力.综述了FACS超高通量酶活性筛选方法的最新研究进展,着重介绍了其在酶定向进化中的应用.     

Regulation of MAPK phosphatase 1 (AtMKP1) by calmodulin in Arabidopsis

The mitogen-activated protein kinases (MAPKs) are key signal transduction molecules, which respond to various external stimuli. The MAPK phosphatases (MKPs) are known to be negative regulators of MAPKs in eukaryotes. We screened an Arabidopsis cDNA library using horseradish peroxidase-conjugated calmodulin (CaM), and isolated AtMKP1 as a CaM-binding protein. Recently, tobacco NtMKP1 and rice OsMKP1, two orthologs of Arabidopsis AtMKP1, were reported to bind CaM via a single putative CaM binding domain (CaMBD). However, little is known about the regulation of phosphatase activity of plant MKP1s by CaM binding. In this study, we identified two Ca(2+)-dependent CaMBDs within AtMKP1. Specific binding of CaM to two different CaMBDs was verified using a gel mobility shift assay, a competition assay with a Ca(2+)/CaM-dependent enzyme, and a split-ubiquitin assay. The peptides for two CaMBDs, CaMBDI and CaMBDII, bound CaM in a Ca(2+)-dependent manner, and the binding affinity of CaMBDII was found to be higher than that of CaMBDI. CaM overlay assays using mutated CaMBDs showed that four amino acids, Trp(453) and Leu(456) in CaMBDI and Trp(678) and Ile(684) in CaMBDII, play a pivotal role in CaM binding. Moreover, the phosphatase activity of AtMKP1 was increased by CaM in a Ca(2+)-dependent manner. Our results suggest that two important signaling pathways, Ca(2+) signaling and the MAPK signaling cascade, are connected in plants via the regulation of AtMKP1 activity. To our knowledge, this is the first report to show that the biochemical activity of MKP1 in plants is regulated by CaM.     

外来植物火炬树(Rhus typhina L.)入侵对不同林型土壤性质的影响

生物入侵在世界范围内广泛发生,严重威胁当地生物多样性和生态系统稳定性。植物与土壤之间的相互作用在决定植物的竞争力以及分布格局中起着重要作用,是影响外来植物入侵力和生态系统可入侵性的一个重要方面。目前,有关研究已成为植被生态学与入侵生态学的研究热点。引自北美的外来植物火炬树(Rhus typhina L.)已成为我国北方主要的入侵木本植物之一。比较了火炬树单优林型、火炬树+刺槐(Robinia pseudoacacia L.)混交林、火炬树+麻栎(Quercus acutissima Carruth.)混交林、火炬树+银白杨(Populus alba L.)混交林4种不同林型的土壤微生物群落结构、土壤酶活性和土壤养分含量特征。结果表明:火炬树单优林土壤细菌、放线菌数量明显高于各混交林型,而真菌数量无显著差异;土壤酶活性方面,火炬树单优林脲酶、过氧化氢酶活性高,土壤磷酸酶活性低;火炬树的入侵显著提高了土壤全碳、全氮、全磷和硝态氮含量,同时明显降低了土壤铵态氮含量。硝态氮含量的增高可能与火炬树入侵造成土壤微生物群落组成变化、土壤硝化速率高有关;而火炬树入侵降低了土壤铵态氮含量,说明该物种可能更易于吸收利用铵态氮。以上研究结果表明,火炬树可以改变土壤生态系统的微生物群落组成和土壤酶活性并影响土壤相关营养元素循环,从而可能使其在与当地植物的竞争中获得优势,为自身的入侵创造有利条件。     

SARS病毒核衣壳蛋白、膜蛋白在大肠杆菌中的高效表达和纯化

通过反转录PCR获得了SARS冠状病毒核衣壳蛋白(N)和膜蛋白(M)基因,其序列分析结果与加拿大多伦多株完全一致。将M基因和N基因克隆到大肠杆菌表达载体pET22b和pBV222上,并在大肠杆菌中以包涵体及可溶形式获得高效表达。通过离子交换、金属螯合层析纯化获得电泳纯制品。所获得的核衣壳蛋白具有良好的抗原性,可用于抗SARS抗体检测及亚单位疫苗研究。     

燕山地区白头翁生境伴生植物资源调查与分析

调查与白头翁共存的伴生植物种类、相似性、生活型、分布区类型等,探讨其生态适应性和地理分布规律,针对性地提出白头翁资源保护利用建议,以期为燕山地区白头翁种质资源的保护和利用提供参考。采用访问调查、路线调查和典型样地调查法,对燕山地区白头翁生境伴生植物进行调查与分析。燕山地区从冀东的秦皇岛地区到冀北的承德地区都有白头翁的分布,多生于向阳的山地草坡上,喜光、耐旱、适于阳生性环境。白头翁生境伴生植物共56科128属164种,主要优势科为菊科（Compositae）、豆科（Leguminosae）、禾本科（Gramineae）、蔷薇科（Rosaceae）、唇形科（Labiatae）、百合科（Liliaceae）、毛茛科（Ranunculaceae）、萝藦科（Asclepiadaceae）等,其中乔木共5科5属7种,灌木共22科38属46种,草本植物共35科85属111种。调查的各样地间相似系数普遍较低,说明燕山地区不同地区白头翁生境差别较大,其伴生植物具有多样性的特点。伴生植物属的分布区类型可分为14个,群落具有明显温带性质。燕山地区白头翁生境多样性及伴生植物的多样性,反映出燕山地区白头翁生态适...     

Regulation of Phospholipase D Activity and Phosphatidic Acid Production after Purinergic (P2Y6) Receptor Stimulation

Phosphatidic acid (PA) is a lipid second messenger located at the intersection of several lipid metabolism and cell signaling events including membrane trafficking, survival, and proliferation. Generation of signaling PA has long been primarily attributed to the activation of phospholipase D (PLD). PLD catalyzes the hydrolysis of phosphatidylcholine into PA. A variety of both receptor-tyrosine kinase and G-protein-coupled receptor stimulations have been shown to lead to PLD activation and PA generation. This study focuses on profiling the PA pool upon P2Y₆ receptor signaling manipulation to determine the major PA producing enzymes. Here we show that PLD, although highly active, is not responsible for the majority of stable PA being produced upon UDP stimulation of the P2Y₆ receptor and that PA levels are tightly regulated. By following PA flux in the cell we show that PLD is involved in an initial increase in PA upon receptor stimulation; however, when PLD is blocked, the cell compensates by increasing PA production from other sources. We further delineate the P2Y₆ signaling pathway showing that phospholipase Cβ3 (PLCβ3), PLCδ1, DGKζ and PLD are all downstream of receptor activation. We also show that DGKζ is a novel negative regulator of PLD activity in this system that occurs through an inhibitory mechanism with PKCα. These results further define the downstream events resulting in PA production in the P2Y₆ receptor signaling pathway.     

A Role for Ifit2 in Restricting West Nile Virus Infection in the Brain

Previous studies have demonstrated that type I interferon (IFN-I) restricts West Nile virus (WNV) replication and pathogenesis in peripheral and central nervous system (CNS) tissues. However, the in vivo role of specific antiviral genes that are induced by IFN-I against WNV infection remains less well characterized. Here, using Ifit2^−/− mice, we defined the antiviral function of the interferon-stimulated gene (ISG) Ifit2 in limiting infection and disease in vivo by a virulent North American strain of WNV. Compared to congenic wild-type controls, Ifit2^−/− mice showed enhanced WNV infection in a tissue-restricted manner, with preferential replication in the CNS of animals lacking Ifit2. Virological analysis of cultured macrophages, dendritic cells, fibroblasts, cerebellar granule cell neurons, and cortical neurons revealed cell type-specific antiviral functions of Ifit2 against WNV. In comparison, small effects of Ifit2 were observed on the induction or magnitude of innate or adaptive immune responses. Our results suggest that Ifit2 restricts WNV infection and pathogenesis in different tissues in a cell type-specific manner.     

乳酸菌载体pMG36e的应用现状

乳酸乳球菌通用表达质粒pMG36e是一个经典的人工构建的组成型表达载体,是以乳酸乳球菌乳脂亚种蛋白酶基因的转录和翻译信号为基础构建而成的。它包含一个强启动子,能够在多种细菌中表达外源蛋白。已用于研究细菌素作用机制,乳酸菌基因工程菌株的改造以及口服疫苗的开发等,应用领域十分广泛,已成为乳酸菌基因工程研究的重要工具质粒之一。本文主要从载体构成、基因表达与食品级载体改造等三方面的应用对其进行综述,旨在为该质粒今后研究提供资料。     

马铃薯杂种F1的SSR鉴定

为选育抗黑痣病、高产优质的马铃薯新品种,选用引进品种‘大西洋’分别与‘陇薯6号’、‘陇薯7号’杂交,获得了杂种F1代,利用SSR标记技术对‘大西洋’与‘陇薯6号’的42个杂种F1、‘大西洋’与‘陇薯7号’的9个杂种F1单株进行了鉴定。从59对SSR引物中筛选出2对在亲本间存在差异、扩增稳定、条带清晰的引物S184和STM1049,用于‘大西洋’ב陇薯6号’杂种F1、‘大西洋’ב陇薯7号’杂种F1及其亲本的基因组DNA扩增。SSR带型分析显示,杂种F1的SSR带型呈双亲互补型、缺失型、父本型和母本型4类,依据带型特征鉴定出供试的51个马铃薯杂种F1单株均为真杂种,表明SSR分子标记技术用于马铃薯杂种真实性鉴定是可行的。该研究可为进一步开展马铃薯杂交后代目标性状优异株系选育提供依据。