红球菌R04联苯/多氯联苯代谢相关调控蛋白RHOGL007659的生理功能

【目的】研究红球菌(Rhodococcus sp.)R04调控蛋白RHOGL007659的生理功能及其缺陷菌株的代谢特性,初步探究红球菌R04降解联苯的调控机制。【方法】通过基因同源重组敲除红球菌R04联苯代谢相关基因RHOGL007659。比较红球菌R04(野生型)和缺陷型菌株R04Δ7659(基因RHOGL007659缺陷型的R04)在不同碳源培养下的生长情况,HPLC分析R04和R04Δ7659转化联苯的能力。提取R04和R04Δ7659的总RNA,实时荧光定量PCR检测联苯降解关键基因的转录表达。纯化Bph B(联苯降解脱氢酶)和Bph D(联苯降解水解酶),制备多克隆抗体。Western blot分析Bph B和Bph D蛋白在R04和R04Δ7659中的表达水平。【结果】获得了RHOGL007659基因的缺陷型菌株R04Δ7659,与R04相比,R04Δ7659在联苯培养条件下的生物量趋近于零。HPLC分析表明,RHOGL007659基因的缺失使红球菌R04丧失转化联苯的能力。实时荧光定量PCR结果表明,在联苯培养条件下,缺失RHOGL007659后的R04,其联苯降解关键基因均有不同程度的下调表达。Western blot分析显示RHOGL007659缺失后,联苯降解关键酶Bph B和Bph D表达量均降低,这与实时荧光定量PCR结果相一致。【结论】RHOGL007659是红球菌R04联苯降解关键基因簇的调控蛋白,该蛋白对红球菌R04代谢联苯过程具有正调控作用。     

嗜吡啶红球菌 R04的联苯降解途径的研究

通过GC-MS测定出嗜吡啶红球菌R04菌降解联苯的中间代谢物2,3二氢二羟基联苯、2,3二羟基联苯和苯甲酸,并测定了该菌的2,3二羟基联苯双加氧酶、2羟基6酮基6苯基2,3己二烯酸(HOPDA)水解酶和苯甲酸双加氧酶活性。最终确定了R04菌降解联苯的途径为2,3二羟基联苯双加氧酶途径。     

B细胞不对称分裂

细胞的不对称分裂对于细胞多样性产生的重要性已经被大部分人所认识。B细胞的不对称分裂首先是在抗体类别转换的研究中发现的。最近,美国5科学家对B细胞在免疫发生中心中不对称分裂的原因进行了探索。结果发表在2012年1月20日出版的《Science》中。B细胞的不对称分裂参与体液免疫的抗体类别转换和抗体亲和力成熟过程。对于其机制仍不清楚,但目前研究初步提示细胞内分子的不对称分布是其发生的上游因素。并且B细胞的不对称分裂可能与不对称抗原分离可能在抗体亲和力成熟过程中具有独立协同作用。     

嗜吡啶红球菌R04的联苯降解途径的研究

通过GC-MS测定出嗜吡啶红球菌R04菌降解联苯的中间代谢物2,3-二氢二羟基联苯、2,3-二羟基联苯和苯甲酸,并测定了该菌的2,3-二羟基联苯双加氧酶、2-羟基-6-酮基-6-苯基-2,3-己二烯酸(HOPDA)水解酶和苯甲酸双加氧酶活性。最终确定了R04菌降解联苯的途径为2,3-二羟基联苯双加氧酶途径。     

红球菌R04苯甲酸转运相关膜蛋白RHOGL009301的生理功能

【目的】探究红球菌(Rhodococcus sp.)R04膜蛋白RHOGL009301的生理功能和突变菌株的代谢特性,确定该膜蛋白的生理功能与苯甲酸转运的关系。【方法】将RHOGL009301基因与绿色荧光蛋白基因在Rhodococcus erythropolis进行融合表达,Delta Vision观察该基因蛋白产物的定位。通过基因同源重组敲除RHOGL009301基因,并对比野生型菌株和缺陷型菌株在不同碳源培养下的生长情况。HPLC测定红球菌R04野生型菌株和缺陷型菌株代谢联苯和苯甲酸时细胞内外代谢物,分析不同生长条件下代谢物的浓度变化。【结果】RHOGL009301基因与绿色荧光蛋白基因在Rhodococcus erythropolis中实现共表达,并定位在细胞膜上。获得了RHOGL009301基因的缺陷型菌株R04ΔMP,与野生型菌株相比,缺陷型菌株在联苯和苯甲酸培养条件下的生物量明显降低,生长速度减慢。HPLC分析表明RHOGL009301基因的缺失抑制了苯甲酸的转运。【结论】膜蛋白RHOGL009301是苯甲酸代谢和转运相关的蛋白,基于序列同源性分析,该膜蛋白是一种新型的苯甲酸转运蛋白。     

神经母细胞：一个干细胞不对称分裂的模型

干细胞自我更新的不对称分裂能产生一个与本身相同的子细胞和一个分化的子细胞。近来通过对神经母细胞（Neuroblast,一组神经干细胞,负责产生中枢神经系统中的多种神经元和胶质细胞）的研究,揭示了干细胞这种自我更新的不对称分裂能力的机制,令人振奋不已。人们发现了几个重要的特异定位的细胞命运决定因子。并探索了它们在细胞骨架重组、细胞周期的进程、细胞质分裂和有丝分裂定向等过程中的分离机制。这些发现为理解干细胞分裂的共同机制提供了有益的启示。     

联苯培养条件下红球菌R04转录表达和苯甲酸代谢途径解析

摘要:【目的】研究不同碳源,特别是联苯条件下红球菌的细胞转录应答,以挖掘与多氯联苯(PCBs)转运、代谢及其调控相关的基因,为进一步全面理解PCB微生物降解的分子机制奠定基础。【方法】以一株多氯联苯降解菌红球菌(Rhodococcus sp.R04)为材料,分别提取不同碳源(乙醇、葡萄糖和联苯)培养条件下菌体的总RNA,反转录合成cDNA。采用高通量测序法分别对这三种样品进行转录组测序,分析测序数据得出全基因组表达模式,并对不同条件下的基因表达进行差示分析,进而对联苯代谢网络和红球菌中其他基因的转录调节和代谢应答反应做出相关性分析。Q-RT-PCR分析不同碳源培养条件下的基因表达情况。【结果】测序结果表明,与葡萄糖和乙醇相比,联苯培养条件下明显上调(log2 Ratio 1)基因个数分别为375和332个。与葡萄糖相比,联苯培养条件下,相关基因上调表达量与Q-RT-PCR实验结果基本一致。功能分类获得细胞组分、分子功能和生物学过程三大类别160多个细小分支的差示表达基因,部分基因参与联苯代谢转录调控、联苯转运、抗氧化应激反应以及信号传导通路系统等多种生理过程。参与联苯上游代谢途径的众多同工酶基因中,只有bphC2和bphD1在联苯中大量上调表达,其余同工酶在联苯中基本量不变或下调表达。转录组注释及差示分析推测,红球菌R04中苯甲酸的代谢主要是通过儿茶酚邻位途径、间位途径以及原儿茶酸途径三条代谢途径完成。【结论】与葡萄糖和乙醇相比,红球菌R04在联苯培养条件下基因表达差异明显,这为我们进一步解析多氯联苯代谢特征和代谢调控提供理论依据。     

杜仲花粉不对称分裂的超微结构观察

运用透射电镜对杜仲花粉发育进程进行了观察研究。结果显示,杜仲小孢子的第一次分裂为不等分裂,形成小的生殖细胞和大的营养细胞。分裂开始前小孢子的营养极形成许多小液泡,建立细胞极性;然后随着核膜的解体核周围的细胞器逐渐向纺锤体区靠近,围绕在纺锤体周围。花粉第一次有丝分裂完成后,生殖细胞所获得的细胞器开始分布在细胞的两侧,后来移向生殖细胞的营养极,而紧贴花粉壁的生殖极无细胞器分布。这种生殖细胞早期的细胞极性,可能为进一步分裂形成精细胞奠定基础。     

哺乳动物卵母细胞不对称分裂的研究进展

哺乳动物卵母细胞成熟过程需要进行两次连续的不对称分裂,最终形成体积差异巨大的子细胞：大体积的卵母细胞和两种体积较小的极体。不对称分裂现象是哺乳动物卵母细胞减数分裂的典型特征,不对称分裂后的卵母细胞是高度极化的细胞。精卵结合后,细胞重新恢复了对称分裂,但是在卵母细胞减数分裂过程中形成的极性特征却得以保留并影响早期胚胎的极性。本文对近年来在哺乳动物卵母细胞不对称分裂方面的相关研究展开综述,从细胞质不对称分裂和细胞核不对称分裂两个方面对染色体、细胞骨架在哺乳动物卵母细胞不对称分裂中的作用、细胞器在哺乳动物卵母细胞成熟过程中的重组分配、染色体非随机分离等过程进行介绍,旨在从细胞和分子水平阐述哺乳动物卵母细胞不对称分裂的主要机制。     

Rhodococcus sp. R04细胞色素P450单加氧酶及CYP125A18与唑类药物的互作分析

红球菌 (Rhodococcus sp.) R04基因组有15种细胞色素P450单加氧酶,其中CYP125A18与结核分枝杆菌 (Mycobacterium tuberculosis) 和马红球菌 (Rhodococcus equi) 的CYP125有较高同源性。利用NCBI蛋白质数据库搜索同源序列,对Rhodococcus sp. R04的15种CYP450一级结构序列进行比对和系统发育分析;对CYP125A18基因进行了克隆表达,并用紫外分光光度法对蛋白质的光谱学特性以及与唑类药物互作情况进行分析。实验结果表明,Rhodococcus sp. R04 15种CYP450均含有保守的氨基酸序列和铁血红素催化中心。SDS-PAGE分析表明,CYP125A18分子量约为50 kD,CYP125A18还原态和CO结合后与CYP125A18氧化态的差示光谱表现为典型的CYP450光谱特性。CYP125A18与底物4-胆甾烯-3-酮结合后,血红素铁全部转变为高自旋状态;与唑类药物滴定后发生了II型光谱转变。解离常数表明,7种唑类药物与CYP125A18的亲和力由强到弱依次为酮康唑、益康唑、4-苯基咪唑、氟康唑、4-甲基-2-苯基咪唑、克霉唑、甲硝唑。上述发现对研究CYP125代谢胆固醇具有重要意义,同时为疾病耐药性研究及药物选择提供数据和理论支持。     

Biodegradation of seven polychlorinated biphenyls by a newly isolated aerobic bacterium (<Emphasis Type="Italic">Rhodococcus</Emphasis> sp. R04)

An aerobic bacterial strain, designated R04, belonging to the genus Rhodococcus has been isolated and characerized by 16S rDNA analysis. The capability of this strain to degrade seven different polychlorinated biphenyls (CBs), 500 ppm 3-CB, 3,4-CB, 4,4-CB, 2,4,6-CB, 2,4,5-CB, 2,3,4,5-CB and 3,4,3,4-CB in liquid medium, was evaluated. After 5 days of incubation, the concentration of chloride increased to 0.35 mM in cultures containing 3-CB and R04, whereas in cultures with 3,4-CB, 2,3,4,5-CB or 3,4,3,4-CB plus R04 the chloride content increased to 0.1 mM. However, non-stoichiometric amounts of chloride were produced in cultures with R04 and 4,4-CB, 2,4,6-CB and 2,4,5-CB. The spectrum of supernatants from R04 grown on seven PCBs had a UV-visible (UV-VIS) absorption at 200–500 nm, characteristic of biphenyl-derived cleavage products. Gas-chromatographic (GC) analysis showed that R04 was able to transform 100% of 3-CB and 3,4-CB after 1 day of incubation, and 95% of 4,4-CB, 2,4,6-CB, 2,4,5-CB, 2,3,4,5-CB and 3,4,3,4-CB after 5 days of incubation. The position of the chlorine substituents on the rings strongly influenced the degradation of polychlorinated biphenyls (PCBs) and their intermediate metabolites by Rhodococcus sp. R04. The degradation of PCBs was further evaluated by monitoring intermediate metabolites of PCBs.     

一株红球菌属细菌LV4在高盐条件下的吡啶降解特性

由微生物介导的吡啶降解技术是解决高盐吡啶环境污染的经济有效方法之一,开发具有吡啶降解性能且能够耐受高盐分的微生物是该类研究的重要前提。本研究从山西太原钢铁公司焦化废水处理厂活性污泥中分离培养了一株耐盐吡啶降解菌,通过菌落形态和16S rDNA基因系统发育分析,鉴定其为红球菌属(Rhodococcus sp.)的细菌。耐盐性实验结果表明,菌株LV4能够在0%–6%盐度范围内生长,并完全降解初始浓度为500 mg/L的吡啶;但当盐度高于4%时,菌株LV4因其生长变缓而导致吡啶完全降解时间明显延长。扫描电镜结果显示,高盐环境会使菌株LV4的菌体细胞分裂变慢,诱导细胞表面分泌更多的颗粒状胞外聚合物(extracellular polymeric substance, EPS)。当盐度不高于4%时菌株LV4主要依靠EPS中蛋白含量的增加来响应高盐环境的冲击。单因素实验优化发现,菌株LV4在盐度为4%的高盐环境中降解吡啶的最佳条件为温度30℃、pH 7.0、转速为120 r/min (DO 10.30 mg/L)。最优条件下菌株LV4对于初始浓度为500 mg/L的吡啶,在经过12 h的适应期后,...     

Removal of benzene and toluene in polyurethane biofilter immobilized with Rhodococcus sp. EH831 under transient loading

The performance of a polyurethane (PU) biofilter inoculated with Rhodococcus sp. EH831 was evaluated under different transient loading conditions, such as shutdown, intermittent and fluctuating loading. A mixture of benzene and toluene vapors was employed as model pollutants. When the biofilter was restarted after a 2 week-shutdown, during which neither clean air nor water was supplied, the benzene and toluene removal capacities were rapidly restored after a re-adaptation period of only 1 day. A comparison of the removal capacity under continuous and intermittent loading revealed that constant and periodic loading (8 h on/16 h off per day) and a 2 day-shutdown did not significantly influence the biofilter performance, although the removals of benzene and toluene were relatively unstable and lower under intermittent loading during the initial week. The result of quantitative real-time PCR showed that Rhodococcus sp. EH831 could be maintained during transient loading periods (10¹⁰–10¹¹ CFU/g-dry PU) irrespective of the different operating conditions.     

Purification, characterization, and substrate specificity of two 2,3-dihydroxybiphenyl 1,2-dioxygenase from Rhodococcus sp. R04, showing their distinct stability at various temperature

The genes of two 2,3-dihydroxybiphenyl 1,2-dioxygenases (BphC1 and BphC2) were obtained from the gene library of Rhodococcus sp. R04. The enzymes have been purified to apparent electrophoretic homogeneity from the cell extracts of the recombinant harboring bphC1 and bphC2. Both BphC1 and BphC2 were hexamers, consisting of six subunits of 35 and 33kDa as determined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, respectively. The enzymes had similar optimal pH (pH 9.0), but different temperatures for their maximum activity (30 degrees C for BphC1, 80 degrees C for BphC2). In addition, they exhibited distinct stability at various temperatures. The enzymes could cleave a wide range of catechols, with 2,3-dihydroxybiphenyl being the optimum substrate for BphC1 and BphC2. BphC1 was inhibited by 2,3-dihydroxybiphenyl, catechol and 3-chlorocatechol, whereas BphC2 showed strong substrate inhibition for all the given substrates. BphC2 exhibited a half-life of 15min at 80 degrees C and 50min at 70 degrees C, making it the most thermostable extradiol dioxygenase studied in mesophilic bacteria. After disruption of bphC1 and bphC2 genes, R04DeltaC1 (bphC1 mutant) delayed the time of their completely eliminating biphenyl another 15h compared with its parent strain R04, but R04DeltaC2 (bphC2 mutant) lost the ability to grow on biphenyl, suggesting that BphC1 plays an assistant role in the degrading of biphenyl by strain R04, while BphC2 is essential for the growth of strain R04 on biphenyl.     

Cloning and expressing DBT (dibenzothiophene) monooxygenase gene (dszC) from Rhodococcus sp. DS-3 in Escherichia coli

Dibenzothiophene (DBT) monooxygenase (DszC) catalysis, the first and also the key step in the microbial DBT desulfurization, is the conversion of DBT to DBT sulfone (DBTO₂). In this study, dszC of a DBT-desulfurizing bacterium Rhodococcus sp. DS-3 was cloned by PCR. The sequence cloned was 99% homologous to Rhodococcus erythropolis IGTS8 that was reported in the Genebank. The gene dszC could be overexpressed effectively after being inserted into plasmid pET28a and transformed into E. coli BL21 strain. The expression amount of DszC was about 20% of total supernatant at low temperature. The soluble DszC in the supernatant was purified by Ni²⁺ chelating His-Tag resin column and sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) to electronics purity. Only one band was detected by Western-blotting, which is for the antibody released in mouse against purified DszC in the expression product of BL21 (DE3, paC5) and Rhodococcus sp. DS-3. The activity of purified DszC was 0.36 U. DszC can utilize the organic compound such as DBT and methyl-DBT, but not DBT derivates such as DBF, which has no sulfur or inorganic sulfur. __________ Translated from Acta Scientiarum Naturalium Universitatis Nankaiensis, 2005, 38(6): 1–6 [译自: 南开大学学报 (自然科学版), 2005, 38(6): 1–6]     

Asymmetric cell division as a route to reduction in cell length and change in cell morphology in trypanosomes

African trypanosomes go through at least five developmental stages during their life cycle. The different cellular forms are classified using morphology, including the order of the nucleus, flagellum and kinetoplast along the anterior-posterior axis of the cell, the predominant cell surface molecules and the location within the host. Here, an asymmetrical cell division cycle that is an integral part of the Trypanosoma brucei life cycle has been characterised in further detail through the use of cell cycle stage specific markers. The cell cycle leading to the asymmetric division includes an exquisitely synchronised mitosis and exchange in relative location of organelles along the anterior-posterior axis of the cell. These events are coupled to a change in cell surface architecture. During the asymmetric division, the behaviour of the new flagellum is consistent with a role in determining the location of the plane of cell division, a function previously characterised in procyclic cells. Thus, the asymmetric cell division cycle provides a mechanism for a change in cell morphology and also an explanation for how a reduction in cell length can occur in a cell shaped by a stable microtubule array.     

Characterization and functional analysis of a novel gene cluster involved in biphenyl degradation in Rhodococcus sp. strain R04

AIMS: Isolation of the genes relative to PCB biodegradation and identification of the bph gene function in Rhodococcus sp. R04. METHODS AND RESULTS: A 8.7-kb fragment carrying the biphenyl catabolic genes bphABCD was isolated from the gene library in Rhodococcus sp. R04. Based on the deduced amino acid sequence homology, seven bph genes, bphA1A2A3A4, bphB, bphC and bphD, were thought to be responsible for the initial four steps of biphenyl degradation. In Escherichia coli, BphA exhibited poor activity for biphenyl transformation, and BphB, BphC and BphD were found to be catalytically active towards 2,3-dihydro-2,3-dihydroxybiphenyl, 2,3-dihydroxybiphenyl and 2-hydroxy-6-oxo-6-phenylhexa-2,4-dienoate, respectively (activities of 50, 8.1 and 2.4 micromol l(-1) min(-1) mg(-1)). SDS-PAGE analysis indicated that the sizes of bphA1A2A3A4, bphB, bphC and bphD gene products were 49, 19, 14, 47, 32, 30 and 31 kDa, respectively. After disruption of bph genes, the bphA1 mutants lost the ability to grow on biphenyl, the bphB and bphD mutants were able to transform a little of biphenyl, but hardly grew on biphenyl. CONCLUSION: The cloned bph genes indeed play an important role in the biphenyl catabolism in this strain. SIGNIFICANCE AND IMPACT OF THE STUDY: This bph gene organization in Rhodococcus sp. R04 differs from that of other biphenyl degraders reported previously, indicating it is a novel type of bph gene cluster. Analysis of the phylogenetic tree suggested that BphA1 and BphA2 in Rhodococcus sp. R04 had a different evolutionary relationship with those in the other PCB degraders.     

Decolourisation of Remazol Brilliant Blue R via a novel Bjerkandera sp. strain

A novel strain of Bjerkandera sp. (B33/3), with particularly high decolourisation activities upon Poly R-478 and Remazol Brilliant Blue R (RBBR) dyes, was isolated. The role of the ligninolytic extracellular enzymes produced by this strain on decolourisation of RBBR was studied in some depth. The basis of decolourisation is an enzyme-mediated process, in which the main enzyme responsible is a recently described peroxidase with capacity for oxidation of manganese, as well as veratryl alcohol and 2,6-dimethoxyphenol in a manganese-independent reaction.