Dihydroartemisinin inhibits plasmid transfer in drug-resistant Escherichia coli via limiting energy supply

Conjugative transfer of antibiotic resistance genes(ARGs)by plasmids is an important route for ARG dissemination.An increasing number of antibiotic and nonantibiotic compounds have been reported to aid the spread of ARGs,highlighting potential challenges for controlling this type of horizontal transfer.Development of conjugation inhibitors that block or delay the transfer of ARG-bearing plasmids is a promising strategy to control the propagation of antibiotic resistance.Although such inhibitors are rare,they typically exhibit relatively high toxicity and low efficacy in vivo and their mechanisms of action are inadequately understood.Here,we studied the effects of dihydroartemisinin(DHA),an artemisinin derivative used to treat malaria,on conjugation.DHA inhibited the conjugation of the IncI2 and IncX4 plasmids carrying the mobile colistin resistance gene(mcr-1)by more than 160-fold in vitro in Escherichia coli,and more than two-fold(IncI2 plasmid)in vivo in a mouse model.It also suppressed the transfer of the IncX3 plasmid carrying the carbapenem resistance gene bla_(NDM-5)by more than twofold in vitro.Detection of intracellular adenosine triphosphate(ATP)and proton motive force(PMF),in combination with transcriptomic and metabolomic analyses,revealed that DHA impaired the function of the electron transport chain(ETC)by inhibiting the tricarboxylic acid(TCA)cycle pathway,thereby disrupting PMF and limiting the availability of intracellular ATP for plasmid conjugative transfer.Furthermore,expression levels of genes related to conjugation and pilus generation were significantly down-regulated during DHA exposure,indicating that the transfer apparatus for conjugation may be inhibited.Our findings provide new insights into the control of antibiotic resistance and the potential use of DHA.

Characterization of a bla_(CTX-M-3),bla_(KPC-2)and bla_(TEM-1B)co-producing IncN plasmid in Escherichia coli of chicken origin

An extensively drug-resistant(XDR)Escherichia coli strain 258E was isolated from an anal swab sample of a chicken farm of Anhui province in China.Genomic analyses indicated that the strain 258E harbors an incompatibility group N(IncN)plasmid pEC258-3,which co-produces bla_(CTX-M-3),bla_(KPC-2),bla_(TEM-1B),qnrS1,aac(6')-Ib-cr,dfrA14,arr-3,and aac(6')-Ib3.Multiple genome arrangement analyses indicated that pEC258-3 is highly homologous with pCRKP-1-KPC discovered in Klebsiella pneumoniae from a patient.Furthermore,conjugation experiments proved that plasmid pEC258-3 can be transferred horizontally and may pose a significant potential threat in animals,community and hospital settings.

嗜酸乳杆菌表达载体的构建及其甘露聚糖酶的表达

为获得产甘露聚糖酶的嗜酸乳杆菌(Lactobacillus acidophilus)菌株,该研究构建甘露聚糖酶表达载体并转化嗜酸乳杆菌,分析重组嗜酸乳杆菌产甘露聚糖酶的酶学性质,并测定重组嗜酸乳杆菌的耐酸性及甘露聚糖酶的抗蛋白酶活性。结果表明,重组嗜酸乳杆菌发酵24 h,其所产甘露聚糖酶活性为353 U/m L。甘露聚糖酶的最适催化pH值为5.5,最适催化温度为55℃。重组嗜酸乳杆菌在pH 2.0~4.5有一定的耐酸性,在pH 2.0条件下2 h的存活率为77.3%。甘露聚糖酶液用胃蛋白酶、胰蛋白酶处理160 min后,甘露聚糖酶的相对酶活分别为65%、28%。表明该甘露聚糖酶具有一定的抗胃蛋白酶和部分抗胰蛋白酶降解能力。

基于全基因组测序的耐多黏菌素和替加环素肺炎克雷伯菌特征研究

目的分析1株多黏菌素和替加环素均耐药的肺炎克雷伯菌基因组特征。方法肺炎克雷伯菌KP2016分离自我院临床痰液标本。采用微量肉汤稀释法测定KP2016对亚胺培南、美罗培南、多黏菌素和替加环素的最低抑菌浓度。对菌株进行第二代Illumina和第三代Oxford Nanopore全基因组测序。通过Unicycler对第二代和第三代序列进行混合拼接。通过ABRicate v0.8.13调用Resfinder数据库分析耐药基因。通过ISFinder分析移动元件。利用CGE(Center for Genomic Epidemiology)网站分析菌株的ST型和质粒复制子类型。利用Proksee对质粒结构进行可视化。结果KP2016菌株对多黏菌素和替加环素均耐药,MIC分别为512和16 mg/L。MLST分析显示KP2016属于ST656,携带多黏菌素耐药相关mcr-1和mcr-8基因和替加环素耐药相关tmexCD1-toprJ1基因簇。KP2016携带1个染色体和5个环形质粒,质粒大小3,991~275,345bp,GC含量44.35%~52.20%。mcr-1基因位于约44kb的质粒p1上,上下游环境为ISKpn26-mcr-1-pap2-ISApl1;mcr-8基因位于IncR/IncN型质粒p2上,遗传结构为ISEcl1-mcr-8-orf-ISKpn26;tmexCD1-toprJ1基因簇结构为IS26-tnfxB1-tmexC1-tmexcD1-toprJ1。此外,菌株还携带多黏菌素耐药相关的染色体介导的CrrB突变(L204V、V237I)。结论肺炎克雷伯菌KP2016多黏菌素耐药由mcr-1、mcr-8和crrB突变介导,替加环素耐药由tmexCD1-toprJ1基因簇介导。应加强合理监测,防止其在医疗机构中进一步传播。

多重耐药弗劳地枸橼酸杆菌的基因组及耐药机制分析

目的对多重耐药弗劳地枸橼酸杆菌进行全基因组分析,为研究其耐药机制提供依据。方法采用含美罗培南的MH培养基对粪便标本进行初筛,经BD Phoenix100全自动微生物鉴定仪进行菌种鉴定及药敏试验,提取耐药菌总DNA进行二代测序和细菌多位点序列分型(MLST),经质粒全基因组序列分析检测质粒的组分和功能,并与参考质粒进行比较,通过质粒接合转移实验分析耐药质粒传递情况。结果413份粪便标本中分离出1株多重耐药弗劳地枸橼酸杆菌,该菌株对头孢菌素类、碳青霉烯类抗菌药物、复方磺胺甲噁唑的耐药率均为100%,对氨曲南、环丙沙星、左氧氟沙星、庆大霉素等抗菌药物呈现不同程度耐药;MLST分型的耐药弗劳地枸橼酸杆菌为ST22型,该菌株共含有5412个基因,含耐药基因367个,包括碳青霉烯酶类耐药基因、AmpC酶基因、大环内酯类耐药基因、氨基糖苷类耐药基、喹诺酮类耐药基因等。质粒的全基因组分析结果显示,该质粒含碳青霉烯类耐药基因blaNDM-1、blaSHV12,该质粒与泄殖腔肠杆菌菌株ECN49质粒和肺炎克雷伯菌菌株质粒pA575-NDM有极高的同源性;质粒接合实验显示,blaNDM-1和blaSHV-12可以通过质粒转移。结论弗劳地枸橼酸杆菌耐药的主要原因之一是含有blaNDM-1、blaSHV-12等耐药基因,并且该耐药性能通过质粒进行水平转移。

NDUFS6蛋白生物信息学分析及过表达质粒的构建与鉴定

目的 应用生物信息学方法分析线粒体呼吸链复合体Ⅰ结构亚基烟酰胺腺嘌呤二核苷酸脱氢酶(泛素)铁硫蛋白6(NDUFS6)的理化性质,构建pCV702-NDUFS6过表达质粒并进行鉴定,为进一步研究NDUFS6蛋白功能奠定基础。方法 利用Expasy、UniProtKB、NCBI、SOPMA等生物信息学工具分析NDUFS6蛋白的理化性质、二级结构等;根据NDUFS6 cDNA序列构建携带NDUFS6基因的过表达质粒pCV702-NDUFS6,转染大鼠心肌细胞H9C2,并设置阴性对照(NC)组和相应空载体CON520作为阳性对照(PC)组,经嘌呤霉素筛选后,采用RT-qPCR和Western blot检测NDUFS6 mRNA和蛋白表达水平。结果 NDUFS6蛋白由116个氨基酸组成,理论等电点pI为9.37。蛋白二级结构以无规则卷曲(占50%)为主。酶切鉴定和基因测序结果显示,pCV702-NDUFS6表达质粒构建成功。RT-qPCR和Western blot结果显示,相较于NC组和PC组,过表达组NDUFS6表达水平均上调(P均<0.05)。结论 成功构建了能在心肌细胞H9C2中有效过表达NDUFS6基因的过表达质粒。

Plasmid DNA Analysis of Pathogenic Escherichia coli in Musk Deer

[Objective] The pathogenic Escherichia coli in musk deer was classified at molecular level to provide basic materials for molecular epidemiology of pathogenic Escherichia coli in musk deer. [Method] Plasmids from 24 pathogenic Escherichia coli in musk deer were extracted by the Lysis Triton method, and then identified by single enzyme digestion with three endonucleases of Hind Ⅲ, EcoR Ⅰ and BamH Ⅰ. [Result] The yield rate of plasmids was 91.6%, and 24 pathogenic Escherichia coli in musk deer had the identical or similar plasmid profiles. [Conclusion] Plasmid DNA analysis offers scientific basis for molecular epidemiology of pathogenic Escherichia coli in musk deer in Sichuan Institute of Musk Deer Breeding.

Researches of Agrobacterium rhizogenes Ri Plasmid rol Genes

Expression of rol genes from Ri plasmid of Agrobacterium rhizogenes not only leads to the excessive formation of adventitious roots, but also exhibits various genetically modified characteristics that have broad prospects for the application of plant genetic improvement. Since the 1980s of the last century, much progress has been made in the studies of A. rhizogenes, in particular the agropine type Ri plasmid rol genes and their applications for plant genetic improvement, which involves the structure and function of Ri plasmid, the characters of rol genes, the influence of rol genes expression on plants growth and development, and the applications of rol genes for genetic improvement of forest tree. In this paper, the advances in this field are reviewed and the existing problems about the application of rol genes for genetic improvement of forest tree are also discussed.

携带bla_(CTX-M)禽大肠杆菌的多重耐药特征和体外致病性研究

【目的】探究携带bla_(CTX-M)禽大肠杆菌的分子流行特点。【方法】检测76株携带bla_(CTX-M)禽大肠杆菌的多重耐药谱、系统进化分群及毒力基因,并分析毒力基因与耐药特点、系统进化分群之间的关联性。【结果】药敏结果显示,携带bla_(CTX-M)禽大肠杆菌对氟苯尼考的耐药率最高,达85.53%(65/76);其次是恩诺沙星,为48.68%(37/76);最常见的多重耐药谱为氟苯尼考+恩诺沙星+乙酰甲喹,达10.53%(8/76)。系统进化分群结果显示,主要的亚群为C群和B1群;其中,C群检出率最高,达53.95%(41/76);其次是B1群,为30.26%(23/76);E群、A群、D群和F群的检出率分别为9.21%(7/76)、2.63%(2/76)、2.63%(2/76)和1.32%(1/76);未检测出B2群和分支I群。毒力基因检测结果显示,76株携带bla_(CTX-M)禽大肠杆菌均检出了至少4种毒力因子,且有11株菌同时携带至少11种毒力基因;其中,有13株菌同时检出禽致病性大肠杆菌(avian pathogenic Escherichia coli,APEC)的5个标志性毒力基因(iroN、iutA、hly、OmpT和iss),检出率为17.11%;有11株菌检出ColV质粒的标志基因(cva/cvi、iroN、iucD/iutA、etsAC、OmpT/hlyF和sitA),检出率为14.47%;有28株菌检出耶尔森菌强毒力岛(high pathogenitility island,HPI)的标志基因irp-2和fyuA,检出率为36.82%。【结论】携带bla_(CTX-M)禽大肠杆菌多为多重耐药菌,且多重耐药菌株携带ColV毒力质粒可能性更高;携带bla_(CTX-M)禽大肠杆菌的多重耐药与致病性有关联,即携带bla_(CTX-M)禽大肠杆菌具有多重耐药的同时,具有致病的可能性更高。

Curing of the Bacillus subtilis Plasmid Using Sodium Dodecyl Sulfate

Curing of Bacillus subtilis plasmid using sodium dodecyl sulfate (SDS)was studied in order to obtain a host strain. An overnight culture of Bacillus subtilis 24/pMX45 was used to inoculate fresh LB containing SDS (0-0.008%). No growth of 24/pMX45 was observed when LB contained an SDS concentration of 0.006% or greater, and the sublethal concentration (w/v) of SDS was 0.005% with a killing rate of 99%. Samples were diluted and plated on LB agar, individual colonies were randomly picked to a selective agar medium by tooth to screen for loss of plasmid-encoded erythomycin resistance. CsCl-EtBr gradient centrifugation and plasmid DNA profile demonstrated that plasmid-cured derivative A7 has completely lost its plasmid. A7 had a shorter lag, and its cell concentration was consistently higher than that of the 24/pMX45. Elimination of the plasmid was first observed after 24/pMX45 had been treated with SDS for 8 h. The percent elimination then continued to increase until about 22 h, after which the fraction of cured cell in the population remained constant. Plasmid cured cell numbers were measured in a separate control culture of 24/pMX45 untreated by SDS. No spontaneous loss of pMX45 was observed after 24/pMX45 were incubated for 24 h and 48 h with shaking at 37 ℃.These results suggested that SDS can be used as curing agent to eliminate the plasmid of Bacillus subtilis.

创伤弧菌溶血素基因vvhA质粒定性标准样品的研制及其在水产品检测中的应用

针对我国缺乏适用于创伤弧菌检测的质粒标准样品的现状,本研究开展了创伤弧菌鉴定即用型定性质粒标准样品的研制和应用工作。首先构建了创伤弧菌毒力基因vvhA的重组质粒,经测序验证后制备成质粒标准样品冻干粉,然后对其进行PCR定性检测及紫外分光光度计法定量分析。均匀性检验结果表明,样品间无显著差异,均匀性良好,符合预期目标;短期稳定性检验结果表明,样品能在4℃、37℃条件下稳定保存14天;长期稳定性检验结果表明,样品能在-20℃条件下稳定保存至少12个月。研究结果表明,创伤弧菌质粒定性标准样品的均匀性和稳定性均符合国家定性标准样品的要求,为创伤弧菌的快速、高通量的定性鉴定分析提供了可靠的参考物质。将标准样品应用于鱼类、贝类等10份海鲜类食品样品的检测中,经传统培养法验证,检测结果准确无误。本研究所研制的创伤弧菌质粒定性标准样品具有较好的商业应用潜力,为其在食品检测领域的推广应用奠定了重要基础。

Construction of the Plasmid Reference Molecule for Detection of Transgenic Soybean MON89788

[Objective] The aim was to construct a plasmid reference molecule (PRM) for detection of transgenic soybean MON89788. [Method] the lectin gene sequence,3'-junction and 5'-junction sequence between host plant DNA integrated DNA of MON89788 soybean were amplified independently,and the three fragments were cloned into the cloning vector pMD18-T in order through molecular manipulation method to construct pMD-LM3M5,the applicability of the constructed novel PRM was tested. [Result] Sequencing confirmation result showed that the PRM was 3 700 bp in length,containing 1 029 bp of recombined DNA fragment. The limits of qualitative detection of the PRM were 10 copies. [Conclusion] The PRM constructed in this study was suitable for the identification of MON89788 event.

停滞棒杆菌遗传改造工具和启动子文库构建

停滞棒杆菌是用于5′-肌苷酸生产的重要微生物底盘。为利用代谢工程技术来创建和优化高效细胞工厂,在停滞棒杆菌中构建遗传改造工具和启动子文库十分必要。本研究使用pCG1复制子构建了大肠杆菌-停滞棒杆菌穿梭载体,建立停滞棒杆菌外源DNA转化方法、基于自杀质粒同源重组的基因敲除方法,最终形成了停滞棒杆菌异源基因稳定表达系统;停滞棒杆菌游离质粒的电转化效率达到(2.3±0.3)×10^(3)cfu/μg;构建停滞棒杆菌的合成启动子文库,筛选得到24个强度差异达30倍的启动子元件,用于停滞棒杆菌中的基因精细表达调控。

FMDV 3D基因真核表达质粒的构建、表达及对Ⅰ型IFN信号通路的作用

本研究旨在构建口蹄疫病毒(Foot-and-mouth disease virus,FMDV)3D基因真核表达质粒,并探究其对Ⅰ型干扰素(interferon,IFN)信号通路的作用。根据GenBank序列合成3D基因并将其插入真核表达载体pXJ41构建真核表达质粒pXJ41-Myc-3D,经PCR、双酶切及测序鉴定正确后分别转染HEK-293T细胞和PK-15细胞,Western blotting及间接免疫荧光试验(indirect immunofluorescence assay,IFA)检测3D蛋白在细胞内的表达及定位。通过双荧光素酶报告基因(Luciferase)、Real-time PCR、TCID50等试验检测HEK-293T细胞中过表达3D蛋白对水疱性口炎病毒(Versicular stomatitis virus,VSV)诱导的Ⅰ型IFN信号通路的影响。结果显示,真核表达质粒pXJ41-Myc-3D构建成功;3D蛋白在HEK-293T细胞中表达,大小约为55 kDa,主要定位在细胞核中;3D蛋白抑制了VSV诱导的IFN-β启动子活性和IFN-β mRNA水平,促进了VSV的复制。本研究为深入探究3D蛋白抑制Ⅰ型IFN信号通路的作用机制奠定了基础。

Uhrf1基因重组腺病毒载体构建及其在小鼠心肌细胞DNA损伤修复中的作用研究

目的:构建携带小鼠泛素样同源域和环指结构域1(Uhrf1)基因的重组腺病毒载体,验证Uhrf1基因在原代乳鼠心肌细胞中的表达情况,并探究其在过氧化氢(H_(2)O2)诱导的心肌细胞DNA损伤中的作用。方法:利用PCR扩增小鼠Uhrf1基因的编码序列,将其酶切后插入pADM-CMV-C-FH载体,获得重组腺病毒质粒ADM-Uhrf1。将该质粒转染至HEK293T细胞包装成重组腺病毒颗粒,数代扩增后进行腺病毒的纯化及滴度检测。分离25只1日龄ICR小鼠原代心肌细胞,分为两组,以感染复数(MOI)为50的比例分别感染ADM-Uhrf1及ADM-control(ADMCtrl),通过Western blot及免疫荧光染色验证重组腺病毒介导的UHRF1蛋白的表达,并利用H_(2)O2诱导心肌细胞DNA损伤,进而探究Uhrf1在DNA损伤修复过程中的作用。结果:通过壳蛋白免疫法检测得到的ADM-Uhrf1病毒滴度为1.8×10^(13) pfu/L。Western blot验证显示UHRF1蛋白表达水平显著升高(P<0.05),免疫荧光染色显示UHRF1主要表达在细胞核内,且Uhrf1的过表达能够显著抑制DNA损伤标志物磷酸化组蛋白H_(2)A变异体(γH_(2)AX)蛋白的表达(P<0.01)。结论:成功构建了携带小鼠Uhrf1基因的重组过表达腺病毒载体,并通过腺病毒递送系统在心肌细胞中实现了Uhrf1的过表达,且Uhrf1的过表达有效减轻了H_(2)O2诱导的心肌细胞DNA损伤。

IGF-1基因克隆及其产物的测序鉴定

基因过表达在基础实验和基因治疗应用中都是常用的手段,而质粒的扩增在基因过表达过程中是不可或缺的技术,如何规范、高效地对质粒进行扩增和提取是基因治疗应用的前提,也是困扰很多基础研究人员的难题。利用现有的实验技术,在降低实验成本基础上,建立过表达质粒扩增、提取的最优方案。首先采用传统方法制作LB培养基和感受态细胞,对转化后的质粒进行大量扩增培养,之后使用商业试剂盒对质粒进行提取,反复试验后对商业试剂盒质粒提取过程进行优化,提高效率,最终获得高纯度和浓度的质粒溶液。经超微量分光光度计、琼脂糖凝胶电泳检测和sanger测序等多种方式检测验证后与NCBI数据库中目标基因序列一致,提示扩增、提取成功。经优化后的质粒扩增、提取方案标准、高效,成本低廉,是质粒基因克隆的最佳选择。

一种诱导表达绿色荧光蛋白穿梭质粒的构建及其在荧光示踪中的应用

细菌的荧光标记是一种重要的常用实验标记技术,用于研究细菌生理生化特性、感染宿主体内示踪、感染细胞示踪等研究。细菌的荧光标记通常通过质粒表达荧光蛋白来实现,而不同类型的细菌,由于菌种特性不同,构建的质粒往往不能通用。本研究构建了一种可诱导表达增强型绿色荧光蛋白的穿梭质粒pBT-iEGFP,该质粒可通过添加无水四环素诱导表达绿色荧光蛋白。诱导表达和传代稳定性试验表明,pBT-iEGFP质粒可在禽致病性大肠杆菌、鼠伤寒沙门菌和马耳他布鲁菌中成功诱导表达绿色荧光蛋白,在五代盲传中该质粒能在细菌中稳定遗传。胞内布鲁菌诱导表达试验证实,pBT-iEGFP质粒可成功示踪细胞感染过程中活的布鲁菌。总之,本研究构建的pBT-iEGFP质粒可作为细菌的荧光示踪研究工具,应用于多种实验研究。

绿色荧光蛋白(GFP)标记杧果细菌性角斑病病原菌及其定殖规律

为研究杧果细菌性角斑病病菌在杧果不同器官组织中的定殖规律。利用电击转化法将质粒pBBR1MCS2-Tac-EGFP导入野油菜黄单胞菌杧果致病变种(Xanthomonas citri pv.mangiferaeindicae)菌株Xcm003中,通过转化子生长表型和外源基因的PCR鉴定,成功获得带绿色荧光蛋白(GFP)标记的转化子Xcm003-EGFP,采用室内刺伤和盆栽苗灌根接种试验,结合组织学观察法,追踪该病原菌在不同杧果器官组织中的定殖规律。结果表明,病原菌通过伤口侵入杧果果实果皮外层细胞层,随着侵染时间推移,向内层果皮细胞层垂直扩散并定殖,后期病原菌在伤口处大量聚集,出现隆起开裂状病斑。在杧果叶片中,病原菌从伤口侵入叶片上表皮细胞层,随后迁移到叶肉细胞间隙,侵染后期,病原菌在气孔和伤口定殖,造成气孔和伤口堵塞,导致接种点出现黑褐色水浸病斑。盆栽苗灌根后发现,该病原菌可在土壤中定殖,入侵杧果根部,但并不扩散至其他杧果组织,不会为害整株幼苗。说明杧果细菌性角斑病病菌可在不同杧果组织中定殖,但仅表现为局部侵染特性。

携带不同耐药基因对耐碳青霉烯类肺炎克雷伯菌适应性及毒力的影响

目的 探讨携带不同耐药基因对耐碳青霉烯类肺炎克雷伯菌(CRKP)的生长适应性及毒力作用的影响。方法 通过PCR方法扩增碳青霉烯类耐药基因(bla_(KPC)、bla_(NDM)、bla_(VIM)、bla_(OXA)、bla_(IMP))及β-内酰胺类耐药基因(bla_(TEM)、bla_(SHV)、bla_(CTX)、bla_(LAP)),测序确定基因型。扩增7个管家基因rpoB、gapA、mdh、pgi、phoE、infB和tonB,测序确定基因型并获得菌株ST类型。根据所携带的碳青霉烯类耐药基因不同,将菌株进行分组,在不同亚胺培南抗生素浓度(0、2、8 mg/mL)下培养细菌,绘制生长曲线,比较各组细菌的生长适应性变化;通过线虫侵染模型用CRKP感染线虫,绘制线虫生存曲线,比较各组细菌对线虫的毒力作用。结果 无抗生素压力下各组菌株生长适应性相似;在2 mg/mL亚胺培南培养基中,双抗性基因组中bla_(KPC)+bla_(NDM)组、bla_(IMP)+bla_(OXA)组生长适应性最强,单抗性基因组中bla_(IMP)组生长适应性最低,差异具有统计学意义(P<0.05)。在8 mg/mL亚胺培南培养基中,双抗性基因组中bla_(KPC)+bla_(NDM)组和bla_(NDM)+bla_(OXA)组生长适应性最强,且分别强于单抗性基因组bla_(KPC)组和bla_(OXA)组;单抗性基因组中bla_(OXA)组生长适应性最弱,bla_(KPC)和bla_(NDM)生长最快,差异具有统计学意义(P<0.05)。在无抗生素压力下,各组菌株对线虫毒力作用有所不同,bla_(KPC)组、bla_(KPC)+bla_(NDM)组和bla_(IMP)+bla_(OXA)组生存曲线右移,线虫中位生存时间延长,菌株毒力减弱;bla_(IMP)+bla_(NDM)组生存曲线左移,线虫中位生存时间缩短,菌株毒力增强,差异具有统计学意义(P<0.05)。结论 携带不同的耐药基因以及携带单个或多个耐药基因均会对菌株的生长适应性和毒力产生不同的影响。

沙眼衣原体质粒编码蛋白3的致病性及免疫保护性研究

目的 探索沙眼衣原体(CT)质粒编码蛋白3(Pgp3)的致病性及免疫保护性。方法 CT L2构建株(GFP)、野生株(WT)和质粒缺失株(PF)分别感染Hela细胞,蛋白质免疫印迹法(Western blotting)和间接免疫荧光法(IFA)检测Pgp3蛋白表达水平;L2 GFP、WT和PF菌株经阴道分别感染C3H小鼠,感染后不同时间点经IFA评估生殖道包涵体形成单位(IFU)数量;组氨酸标记的Pgp3(His-Pgp3)体外刺激人输卵管上皮细胞,24 h后经Hoechst 33 528染色和流式细胞术检测细胞凋亡情况;L2 WT体外感染L929和L929-Pgp3细胞,在感染后30、60及80 h固定细胞并计算IFU和细胞核数量。L2 GFP和WT菌株经阴道分别感染C3H小鼠,50 d后各组均以L2 WT菌株攻毒,攻毒后不同时间点评估生殖道IFU数量。结果 L2 GFP Pgp3蛋白表达水平高于L2 WT,L2 PF无Pgp3蛋白表达;小鼠感染后第3、7、10和14天,L2 GFP感染组IFU数量显著高于L2 WT和L2 PF感染组,且L2 GFP组感染周期最长;Pgp3体外干预组细胞凋亡率显著低于空白组,L2 WT体外感染L929和L929-Pgp3细胞60 h和80 h后,L929-Pgp3组IFU值显著高于L929组,且宿主细胞消亡数量显著低于L929组;动物实验显示L2 GFP组经L2 WT菌株攻毒后下生殖道IFU数量显著低于L2 WT组,且L2 GFP组感染周期显著短于L2 WT组。结论 Pgp3可抑制宿主细胞凋亡并促进CT在细胞间播散感染;内源性Pgp3有良好的免疫保护性。