Periplasmic proteins of Escherichia coli are highly resistant to aggregation: reappraisal for roles of molecular chaperones in periplasm

Periplasmic proteins of Gram-negative bacteria like Escherichia coli are subjected to immediate affect of environmental fluctuation that may unfold proteins, due to the permeability of the outer membrane to small molecules. They are thus supposedly protected by certain molecular chaperones. Nevertheless, no homologues of typical molecular chaperones have so far been found in periplasm, and the recently reported chaperone activities of periplasmic protein disulfide isomerase (PDI) and peptidyl prolyl isomerase (PPI) seem to be too weak to satisfy such assumed needs. In an attempt to reveal whether periplasmic proteins exhibit certain unusual properties, we discovered that such proteins as a whole are highly resistant to aggregation under a wide variety of denaturing conditions. Furthermore, in an effort to unveil the nature behind this phenomenon we purified and examined four prominent periplasmic proteins. Our results demonstrate that these proteins unfold at rather mild denaturing conditions and expose hydrophobic surfaces during such unfolding process, but hardly form complexes with a typical molecular chaperone. Based on these observations, we propose that the periplasmic proteins have been evolved to resist the formation of aggregates when subjected to various denaturing conditions and molecular chaperones may thus not be needed in periplasm.     

Steady-state,Pre-steady-state,and Single-turnover Kinetic Measurement for DNA Glycosylase Activity

Human 8-oxoguanine DNA glycosylase (OGG1) excises the mutagenic oxidative DNA lesion 8-oxo-7,8-dihydroguanine (8-oxoG) from DNA. Kinetic characterization of OGG1 is undertaken to measure the rates of 8-oxoG excision and product release. When the OGG1 concentration is lower than substrate DNA, time courses of product formation are biphasic; a rapid exponential phase (i.e. burst) of product formation is followed by a linear steady-state phase. The initial burst of product formation corresponds to the concentration of enzyme properly engaged on the substrate, and the burst amplitude depends on the concentration of enzyme. The first-order rate constant of the burst corresponds to the intrinsic rate of 8-oxoG excision and the slower steady-state rate measures the rate of product release (product DNA dissociation rate constant, k_off). Here, we describe steady-state, pre-steady-state, and single-turnover approaches to isolate and measure specific steps during OGG1 catalytic cycling. A fluorescent labeled lesion-containing oligonucleotide and purified OGG1 are used to facilitate precise kinetic measurements. Since low enzyme concentrations are used to make steady-state measurements, manual mixing of reagents and quenching of the reaction can be performed to ascertain the steady-state rate (k_off). Additionally, extrapolation of the steady-state rate to a point on the ordinate at zero time indicates that a burst of product formation occurred during the first turnover (i.e. y-intercept is positive). The first-order rate constant of the exponential burst phase can be measured using a rapid mixing and quenching technique that examines the amount of product formed at short time intervals (<1 sec) before the steady-state phase and corresponds to the rate of 8-oxoG excision (i.e. chemistry). The chemical step can also be measured using a single-turnover approach where catalytic cycling is prevented by saturating substrate DNA with enzyme (E>S). These approaches can measure elementary rate constants that influence the efficiency of removal of a DNA lesion.     

Genetic diversity and its relationship to hybrid performance in maize as revealed by RFLP and AFLP markers

 The challenge to maize breeders is to identify inbred lines that produce highly heterotic hybrids. In the present study we surveyed genetic divergence among 13 inbred lines of maize using DNA markers and assessed the relationship between genetic distance and hybrid performance in a diallel set of crosses between them. The parental lines were assayed for DNA polymorphism using 135 restriction fragment length polymorphisms (RFLPs) and 209 amplified-fragment polymorphisms (AFLPs). Considerable variation among inbreds was detected with RFLP and AFLP markers. Moreover AFLPs detect polymorphisms more efficiently in comparison to RFLPs, due to the larger number of loci assayed in a single PCR reaction. Genetic distances (GDs), calculated from RFLP and AFLP data, were greater among lines belonging to different heterotic groups compared to those calculated from lines of the same heterotic group. Cluster analysis based on GDs revealed associations among lines which agree with expectations based on pedigree information. The GD values of the 78 F₁ crosses were partioned into general (GGD) and specific (SGD) components. Correlations of GD with F₁ performance for grain yield were positive but too small to be of predictive value. The correlations of SGDs, particularly those based on AFLP data, with specific combining-ability effects for yield may have a practical utility in predicting hybrid performance. Received: 15 August 1997 / Accepted: 19 September 1997     

基于2个核糖体DNA序列的国产白酒草属、小舌菊属和歧伞菊属(菊科紫菀族)分子系统学研究(英文)

国产白酒草亚族(菊科紫菀族)由白酒草属(Conyza)、小舌菊属(Microglossa)和歧伞菊属(Thespis)3个小属组成,且国产白酒草亚族各属间及其与非洲白酒草属植物之间的分子系统发育关系尚无报道,故本研究利用核糖体DNA ITS和ETS序列并采用最大简约法和贝叶斯分析法,重建了国产白酒草亚族的分子系统发育树。结果表明,国产4种白酒草属植物、歧伞菊和非洲白酒草属植物组成一支,而劲直白酒草的两变种和小舌菊嵌入田基黄亚族分支;小舌菊与Psiadia pascalii近缘。基于这些结果,我们认为:(1)劲直白酒草和Conyza incisa应处理为田基黄亚族的一个独立的属;(2)国产4种白酒草属植物和歧伞菊以及大多数非洲白酒草属植物属于Eschenbachia属,而且Eschenbachia属代表一个新的亚族,歧伞菊可处理为Eschenbachia属的一个组。Eschenbachia属可能从非洲经数次长距离传播到达我国南部;(3)Welwitschiella和小舌菊属应保持属的地位,Psiadia pascalii、Conyza scabrida和C.pyrrhopappa可并入小舌菊属。     

月季遗传资源的评价与利用

国产蔷薇属植物82种,约占世界总数的41%.在近200种蔷薇属植物中,只有15种参与了现代月季的形成,新的遗传资源的引入是月季抗性育种的关键.现代月季品种达25000多个,但在欧洲苗圃销售的不到3000个,而以丰花月季为主.月季抗病遗传资源的研究主要针对黑斑病、白粉病和根结线虫.分子标记已广泛应用于月季亲缘关系分析、遗传图谱的构建和品种的鉴定.蔷薇果含有丰富的Vc和药用价值.     

Injected mitotic extracts induce condensation of interphase chromatin

Although extracts from mitotic cells have been shown to induce chromosome condensation when injected into amphibian oocytes, they have not as yet been shown to induce this response in somatic interphase cells. In the experiments reported here, when mitotic extracts were injected into syncytial frog embryos, whose somatic nuclei were arrested in interphase, chromosome condensation was observed. The inability of interphase extracts, injected at similar concentrations, to induce this event demonstrates the cell cycle-specific accumulation of the factors responsible.     

中国近海牡蛎系统分类研究的现状和对策

探讨了中国近海沿岸牡蛎分类的诸多疑难和热点问题,回顾了国内外包括贝类等动物的分子系统发生学研究的主要进展,分析了中国近海牡蛎系统分类目前存在的问题,重点阐述了利用分子标记等手段解决形态相似种的鉴定和种系发生关系等问题的巨大潜力,报道了利用分子标记进行牡蛎分类研究所取得的最新进展。预期经典分类学和分子系统发生学研究的交叉综合,将大力推动中国近海牡蛎的系统分类和系统发生研究的发展。     

上海市进口火龙果软腐病病害分析

应用病原形态学和真菌rDNA-ITS分子标记及Fusarium oxysporum种特异性序列分析, 对引起上海市水果市场销售的进口火龙果软腐的市场病害进行了分离与鉴定, 明确了两种主要的致病真菌为尖孢镰刀菌(Fusarium oxysporum)和单隔镰刀菌(Fusarium dimerum)。其中, F. oxysporum为引起进口火龙果采后软腐的最主要病原真菌, 该菌最适生长温度和致病温度均为25 °C, 光照条件下的致病性强, 在15 °C和35 °C条件下致病性明显降低, 5 °C和45 °C条件下该菌无法正常生长和致病, 并且该菌还能够引起香蕉、番茄、葡萄等多种水果腐烂。系统研究引起进口火龙果采后软腐病病原真菌的生物学特性, 为进口火龙果采后病原真菌有效控制方法的制定提供了有益的参考。     

Specific identification and molecular typing analysis of Lactobacillus johnsonii by using PCR-based methods and pulsed-field gel electrophoresis

A fast and reliable Multiplex-PCR assay was established to identify the species Lactobacillus johnsonii. Two opposing rRNA gene-targeted primers have been designed for this specific PCR detection. Specificity was verified with DNA samples isolated from different lactic acid bacteria. Out of 47 Lactobacillus strains isolated from different environments, 16 were identified as L. johnsonii by PCR. The same set of strains was investigated with five alternative molecular typing methods: enterobacterial repetitive intergenic consensus PCR (ERIC-PCR), repetitive extragenic palindromic PCR (REP-PCR), amplified fragment length polymorphism, single triplicate arbitrarily primed PCR, and pulsed-field gel electrophoresis in order to compare the discriminatory power of these methods. The reported data strongly support the highly significant heterogeneity among all L. johnsonii isolates, potentially linked to their origin of isolation. The use of species-specific primers as well as rapid and highly powerful PCR-based molecular typing tools (namely ERIC- and REP-PCR techniques) should be respectively envisaged for identifying, differentiating and monitoring L. johnsonii strains from various environmental samples, for product monitoring, for species tracing in clinical studies as well as bacterial profiling of various microecological or gastrointestinal environments.     

水稻淀粉合成的分子生物学研究进展

本文综述了水稻淀粉合成的分子生物学研究的最新进展,主要内容是参与淀粉合成的酶鉴定及其基因表达调控,也介绍了对这些酶的遗传操作改良稻米淀粉品质等内容