耐辐射奇球菌dps突变株的构建和蛋白功能初步研究

Dps(DNAprotection during starvation)蛋白是原核生物中特有的一类具有铁离子结合和抗氧化损伤功能的重要蛋白。利用体外PCR扩增技术和体内同源重组方法,获得了耐辐射奇球菌(Deinococcus radiodurans)dps全基因(DRB0092)缺失突变株。对突变株和野生型分别进行不同浓度过氧化氢(H2O2)处理,结果表明:与野生型菌株R1相比,dps突变株在低浓度H2O2(≤10mmol/L)条件下存活率急剧下降,而高浓度(≥30mmol/L)下则完全致死。Native-PAGE活性染色结果显示,稳定生长期dps突变株体内两种过氧化氢酶(KatA和KatB)的活性较野生型R1分别上调2.3倍和2.6倍。通过质粒构建和大肠杆菌诱导表达,获得可溶性Dps蛋白。体外结合和DNA保护实验结果显示:Dps具有明显的DNA结合功能,并能保护质粒DNA免受羟自由基攻击。本研究证明,Dps蛋白在耐辐射奇球菌抗氧化体系中发挥重要作用,可能对该菌极端抗性机制有重要贡献。     

耐辐射奇球菌crtⅠ基因缺失突变株的构建及其功能研究

利用PCR方法和体内同源重组技术,对耐辐射奇球菌(Deinococcus radiodurans)中控制色素合成的关键基因--crtⅠ进行缺失突变,成功获得红色色素缺失突变株M61.对突变株分别进行不同剂量电离辐射(IR)和不同浓度过氧化氢(H2O2)处理,结果表明与野生型菌株R1相比,突变株M61对电离辐射的抗性降低;对过氧化氢的敏感性明显上升,在高浓度H2O2条件下表现异常敏感.HPLC分析结果显示,crtⅠ基因的完全缺失对色素合成途径产生重要影响,导致番茄红素和其他红色类胡萝卜素的合成被抑制.证明crtⅠ基因是耐辐射奇球菌中控制红色类胡萝卜素合成的一个关键基因.为阐明耐辐射奇球菌中类胡萝卜素参与的抗辐射和抗氧化机制奠定了一定基础,为进一步研究类胡萝卜素在耐辐射奇球菌中的合成途径及功能提供了思路.     

耐辐射奇球菌crtI基因缺失突变株的构建及其功能研究

利用PCR方法和体内同源重组技术,对耐辐射奇球菌(Deinococcus radiodurans)中控制色素合成的关键基因———crtI进行缺失突变,成功获得红色色素缺失突变株M61。对突变株分别进行不同剂量电离辐射(IR)和不同浓度过氧化氢(H2O2)处理,结果表明:与野生型菌株R1相比,突变株M61对电离辐射的抗性降低;对过氧化氢的敏感性明显上升,在高浓度H2O2条件下表现异常敏感。HPLC分析结果显示,crtI基因的完全缺失对色素合成途径产生重要影响,导致番茄红素和其他红色类胡萝卜素的合成被抑制。证明crtI基因是耐辐射奇球菌中控制红色类胡萝卜素合成的一个关键基因。为阐明耐辐射奇球菌中类胡萝卜素参与的抗辐射和抗氧化机制奠定了一定基础,为进一步研究类胡萝卜素在耐辐射奇球菌中的合成途径及功能提供了思路。     

耐辐射球菌基因DR1709与DR2523的突变分析

摘要：【目的】检测在耐辐射球菌抵抗外来辐射和氧自由基的过程中,锰离子转运蛋白基因（DR1709和DR2523）是否发挥了作用。探讨锰离子、锰离子转运蛋白基因与耐辐射球菌辐射抗性之间的关系。【方法】分别构建这两个基因的突变体。对突变体和野生型进行紫外线照射和过氧化氢处理。对处理后的菌株存活率进行分析。【结果】DR2523被突变以后,耐辐射球菌在tryptone-glucose-yeast extract (TGY)培养液中的生长受影响很小。而DR1709突变体M1709在对数生长阶段的生长速度远低于野生型。     

耐辐射球菌recQ双突变株的构建及逆境分析

RecQ解螺旋酶是生物有机体在进化中高度保守的SF1超级家族解螺旋酶的一个亚族,它对维持基因组的稳定性有重要的作用。耐辐射球菌野生型菌株R1有两个具有特殊结构的解螺旋酶DR1289和DR2444,运用PCR突变法克隆具有自身groEL启动子、KAT启动子与卡那霉素抗性基因、氯霉素抗性基因融合的DNA片段反向重组到基因组中,首次构建并鉴定了卡那霉素抗性完全突变株ΔDR1289,氯霉素抗性完全突变株ΔDR2444,双突变株ΔrecQ。辐射条件下和H2O2氧化压力下突变株生存率结果表明:ΔDR2444与R1存活率趋势线基本一致,而ΔDR1289和ΔrecQ双突变株较为敏感。根据上述结果推测,DR1289是一个对R1保持极端抗性的必须基因,而DR2444则是极端抗性的非必须基因。     

耐辐射奇球菌dps突变株的构建和蛋白功能初步研究

Dps(DNAprotection during starvation)蛋白是原核生物中特有的一类具有铁离子结合和抗氧化损伤功能的重要蛋白。利用体外PCR扩增技术和体内同源重组方法,获得了耐辐射奇球菌(Deinococcus radiodurans)dps全基因(DRB0092)缺失突变株。对突变株和野生型分别进行不同浓度过氧化氢(H₂O₂)处理,结果表明:与野生型菌株R1相比,dps突变株在低浓度H₂O₂(≤10mmol/L)条件下存活率急剧下降,而高浓度(≥30mmol/L)下则完全致死。Native-PAGE活性染色结果显示,稳定生长期dps突变株体内两种过氧化氢酶(KatA和KatB)的活性较野生型R1分别上调2.3倍和2.6倍。通过质粒构建和大肠杆菌诱导表达,获得可溶性Dps蛋白。体外结合和DNA保护实验结果显示:Dps具有明显的DNA结合功能,并能保护质粒DNA免受羟自由基攻击。本研究证明,Dps蛋白在耐辐射奇球菌抗氧化体系中发挥重要作用,可能对该菌极端抗性机制有重要贡献。     

耐辐射奇球菌辐射损伤修复机制的研究进展

耐辐射奇球菌是迄今为止发现的对辐射抗性最强的原核生物,是研究DNA损伤与修复的模式生物.耐辐射奇球菌(Deinococcus radiodurans,DR)对于电离辐射、紫外线、干燥、H2O2以及其他一些DNA损伤剂均表现出极强的抵抗能力,对于这种超强抗性的具体机制,学界至今尚未形成定论.对DR DNA损伤修复机制的解释包括切除修复和重组修复.本文就耐辐射奇球菌DNA辐射损伤后修复机制的研究进展作一综述.     

耐辐射球菌RNA聚合酶β亚基突变对基因表达全局的影响

RNA聚合酶的B亚基参与与利福平的结合,并在原核生物中高度保守．许多细菌中利福平耐药株的rpoB基因均有氨基酸改变．本实验室曾分离2两株耐辐射球菌（Deinococcus radiodurans）自发突变利福平耐药株（突变为：L420R和1258—669-bp缺失）．本研究发现,β亚基的变化对生长速度有独特的效果．利用DNA芯片技术和生化分析鉴定耐辐射球菌的利福平突变株如何调控基因表达改变生长速度的分子机制．参与代谢、细胞进程和信号传递以及信息贮存和处理的基因的转录在9bp缺失突变株中显著改变．9bp缺失突变株的上调基因的共有启动子序列为富含AT的序列．与野生株相比,L420R和9bp缺失突变株积聚了更多的活性自由基．这些结果初步探讨了D亚基突变调控基因的表达机制．     

PprⅠ和RecⅩ蛋白对耐辐射奇球菌抗氧化作用的影响

利用基因突变、化学发光法和酶活性分析研究了耐辐射奇球菌中与辐射抗性密切相关的基因pprⅠ(Dr0167)和recⅩ(Dr1310)突变对菌体活性氧清除作用的影响,分析了其对抗氧化酶活性的调控功能.实验结果表明,缺失pprⅠ的突变株对活性氧自由基氧化异常敏感,过氧化氢酶和超氧化物歧化酶活性显著降低.与之相反,RecⅩ对菌体活性氧清除作用表现为一种"负"的影响,即缺失recⅩ的突变株对活性氧自由基的清除能力反而增强了,过氧化氢酶和超氧化物歧化酶的酶活性明显增加.表明这两个基因与抗氧化系统的调控有关.为进一步研究该菌的抗氧化机制提供了一些思路.     

PprI和RecX蛋白对耐辐射奇球菌抗氧化作用的影响

利用基因突变、化学发光法和酶活性分析研究了耐辐射奇球菌中与辐射抗性密切相关的基因pprI(Dr0167)和recX(Dr1310)突变对菌体活性氧清除作用的影响,分析了其对抗氧化酶活性的调控功能。实验结果表明,缺失pprI的突变株对活性氧自由基氧化异常敏感,过氧化氢酶和超氧化物歧化酶活性显著降低。与之相反,RecX对菌体活性氧清除作用表现为一种“负”的影响,即缺失recX的突变株对活性氧自由基的清除能力反而增强了,过氧化氢酶和超氧化物歧化酶的酶活性明显增加。表明这两个基因与抗氧化系统的调控有关。为进一步研究该菌的抗氧化机制提供了一些思路。     

ATP-type DNA ligase requires other proteins for its activity in vitro and its operon components for radiation resistance in Deinococcus radiodurans in vivo

A multiprotein DNA processing complex isolated from Deinococcus radiodurans contains the DNA repair protein PprA, an ATP-type DNA repair ligase (LigB) encoded by the drB0100 gene, and protein kinase activity. An ATP-dependent DNA end-joining activity was detected in the complex. To elucidate the function of the drB0100 gene, we generated the deletion mutant for the DR_B0100 ORF. The mutant exhibited a nearly 2-log cycle reduction in growth rate when exposed to a 10,000 Gray dose of γ-radiation, and a significant loss in mitomycin C and methylmethane sulphonate tolerance as compared with wild type. Functional complementation of these phenotypes required the wild-type copy of drB0100 along with other genes such as drb0099 and drb0098, organized downstream in the operon. The in vitro DNA ligase activity of LigB was stimulated severalfold by PprA in the presence of the recombinant DRB0098 protein. However, this activity did not improve when PprA was substituted with purified DRB0099 protein or when DRB0098 protein was substituted with the DRB0099 protein in the presence of PprA in solution. These results suggest that PprA and DRB0098 protein are required for LigB function. Furthermore, they also suggest that the LigB operon components contribute to radiation resistance and double-strand break (DSB) repair in D. radiodurans.     

Evaluation of the antioxidant effects of carotenoids from Deinococcus radiodurans through targeted mutagenesis, chemiluminescence, and DNA damage analyses

Deinococcus radiodurans is highly resistant to reactive oxygen species (ROS). The antioxidant effect of carotenoids in D. radiodurans was investigated by using a targeted mutation of the phytoene synthase gene to block the carotenoid synthesis pathway and by evaluating the survival of cells under environmental stresses. The colorless mutant R1DeltacrtB of D. radiodurans failed to synthesize carotenoids, and was more sensitive to ionizing radiation, hydrogen peroxide, and desiccation than the wild type, suggesting that carotenoids in D. radiodurans help in combating environmental stresses. Chemiluminescence analyses showed that deinoxanthin, a major product in the carotenoid synthesis pathway, had significantly stronger scavenging ability on H2O2 and singlet oxygen than two carotenes (lycopene and beta-carotene) and two xanthophylls (zeaxanthin and lutein). Deinoxanthin also exhibited protective effect on DNA. Our findings suggest that the stronger antioxidant effect of deinoxanthin contribute to the resistance of D. radiodurans. The higher antioxidant effect of deinoxanthin may be attributed to its distinct chemical structure which has an extended conjugated double bonds and the presence of a hydroxyl group at C-1' position, compared with other tested carotenoids.     

RecBC enzyme overproduction affects UV and gamma radiation survival of Deinococcus radiodurans

Deinococcus radiodurans recovering from the effect of acute dose of gamma (gamma) radiation shows a biphasic mechanism of DNA double strands breaks repair that involves an efficient homologous recombination. However, it shows higher sensitivity to near-UV (NUV) than Escherichia coli and lacks RecBC, a DNA strand break (DSB) repair enzyme in some bacteria. Recombinant Deinococcus expressing the recBC genes of E. coli showed nearly three-fold improvements in near-UV tolerance and nearly 2 log cycle reductions in wild type gamma radiation resistance. RecBC over expression effect on radiation response of D. radiodurans was independent of indigenous RecD. Loss of gamma radiation tolerance was attributed to the enhanced rate of in vivo degradation of radiation damaged DNA and delayed kinetics of DSB repair during post-irradiation recovery. RecBC expressing cells of Deinococcus showed wild type response to Far-UV. These results suggest that the overproduction of RecBC competes with the indigenous mechanism of gamma radiation damaged DNA repair while it supports near-UV tolerance in D. radiodurans.     

DNA-membrane complex restoration in Micrococcus radiodurans after X-irradiation: relation to repair, DNA synthesis and DNA degradation

The DNA-membrane complex in Micrococcus radiodurans was shown to be essentially constituted of proteins, lipids and DNA. The complex was dissociated immediately after X-irradiation of cells and restored during post-incubation in complete medium. In X-irradiated protoplasts some DNA remained associated with the complex. Restoration of the complex during post-incubation was only seen in a medium favouring DNA polymerase and ligase activities. Under this condition no DNA synthesis occurred, suggesting that complex restoration may involve ligase activity. The complex restoration in the wild type and the X-ray sensitive mutant UV17 of M. radiodurans was strictly dependent on the X-ray dose. It was correlated with survival and DNA degradation but always preceded the onset of DNA synthesis after X-irradiation. At the same dose the complex restoration was about 2 fold lower in mutant than in wild type cells indicating that the restoration of the complex is related to repair capacity. The results are consistent with the idea that the complex protects X-irradiated DNA of M. radiodurans from further breakdown and, subsequently, permits DNA synthesis and repair to occur.     

The DNA excision repair system of the highly radioresistant bacterium Deinococcus radiodurans is facilitated by the pentose phosphate pathway

Deinococcus radiodurans is highly resistant to radiation and mutagenic chemicals. Mutants defective in the putative glucose-6-phosphate dehydrogenase gene (zwf-) and the aldolase gene (fda-) were generated by homologous recombination. These mutants were used to test the cells' resistance to agents that cause dimer formation and DNA strand breaks. The zwf - mutants were more sensitive to agents that induce DNA excision repair, such as UV irradiation and H2O2, but were as resistant to DNA strand break-causing agents such as methylmethanesulphonic acid (MMS) and mitomycin C (MMC) as the wild-type cells. Analysis of the cytoplasmic fraction of zwf- cells showed that the concentrations of inosine monophosphate (IMP) and uridine monophosphate (UMP) were only 30% of those found in the wild-type cells. The fda- mutants were slightly more resistant to UV light and H2O2. Results suggested that the deinococcal pentose phosphate pathway augmented the DNA excision repair system by providing cells with adequate metabolites for the DNA mismatch repair.     

Identification, sequencing, and targeted mutagenesis of a DNA polymerase gene required for the extreme radioresistance of Deinococcus radiodurans.

Deinococcus radiodurans and other species of the same genus share extreme resistance to ionizing radiation and many other agents that damage DNA. Two different DNA damage-sensitive strains generated by chemical mutagenesis were found to be defective in a gene that has extended DNA and protein sequence homology with polA of Escherichia coli. Both mutant strains lacked DNA polymerase, as measured in activity gels. Transformation of this gene from wild-type D. radiodurans restored to the mutants both polymerase activity and DNA damage resistance. A technique for targeted insertional mutagenesis in D. radiodurans is presented. This technique was employed to construct a pol mutant isogenic with the wild type (the first example of targeted mutagenesis in this eubacterial family). This insertional mutant lacked DNA polymerase activity and was even more sensitive to DNA damage than the mutants derived by chemical mutagenesis. In the case of ionizing radiation, the survival of the wild type after receiving 1 Mrad was 100% while survival of the insertional mutant extrapolated to 10(-24). These results demonstrate that the gene described here encodes a DNA polymerase and that defects in this pol gene cause a dramatic loss of resistance of D. radiodurans to DNA damage.     

Resistance of Deinococcus radiodurans to Mutagenesis Is Facilitated by Pentose Phosphate Pathway in the mutS1 Mutant Background

MutS1 is a key protein involved in mismatch repair system for ensuring fidelity of replication and recombination in Deinococcus radiodurans. The zwf gene encodes glucose-6-phosphate dehydrogenase (G6PD) in the pentose phosphate (PP) pathway, which provides adequate metabolites as precursors of DNA repair. In this study, mutS1 and zwf were disrupted by homologous recombination. The zwf mutant (Deltazwf) and the zwf/mutS1 double mutant (Deltazwf/mutS1) were sensitive to ultraviolet (UV) light, H(2)O(2), and DNA cross-linking agent mitomycin C (MMC), whereas the mutS1 mutant (DeltamutS1) showed resistance to UV light, H(2)O(2) and MMC as the wild-type strain. Inactivation of mutS1 resulted in a 3.3-fold increase in frequency of spontaneous rifampicin-resistant mutagenesis and a 4.9-fold increment in integration efficiency of a donor point-mutation marker during bacterial transformation. Although inactivation of zwf had no obvious effect compared with the wild-type strain, dual disruption of zwf and mutS1 resulted in a 4.7-fold increase in mutation frequency and a 7.4-fold increase in integration efficiency. These results suggest that inactivation of the PP pathway decreases the resistance of D. radiodurans cells to DNA damaging agents and increases mutation frequency and integration efficiency in the mutS1 mutant background.