Identification of E. coli K12 chromosomal insertion sites of bacteriophage φ297

Objective:To identify the specific integration site of prophage φ297 in the host of E. coli K12 chromosome. Methods:Using molecular techniques such as Siebert PCR for walking from the int gene of prophage 297, which is similar to that of phage 933W to an unknown region in genomic DNA. A special adaptor is ligated to the ends of DNA fragments generated by digestion of genomic DNA with restriction enzymes that generates blunt ended fragments. Clone and subclone of PCR products, DNA sequencing and data analysis were used in this study. Results:The attL, attR and the core sequences were determined. The bacterial attachment site of phage φ297 was located in the yecE gene of E. coli K12. Conclusion:The phage φ297 integrates into the yecE gene of the E. coli K12 genome.

Characteristics of β-Lactamase Synthesis in E. coli and K. pneumanie Strains in Nosocomial Infections

Background: Recently micro-organisms that synthesize extended-spectrum β-lactamase (ESBLs) were increased. The peculiarities of ESBL synthesis of Escherichia coli and Klebsiella pneumoniae strains that cause nosocomial urinary tract infections, surgical site infections and pneumonia in surgical clinic were studied. ESBL synthesis were observed 38.9% of E. coli strains obtained from urine, 92.3% of strains obtained from surgical site infections, and 50% of strains obtained from sputum. ESBL synthesis were observed 37.5% of K. pneumoniae strains obtained from urine, 85.7% of strains obtained from surgical site infections, and 60% of strains obtained from sputum. Different levels of ESBL synthesize of E. coli and K. pneumoniae strains isolated from different pattern is discussed. Conclusion. ESBL synthesis is common in E. coli and K. pneumoniae strains, which cause nosocomial infections. The frequency of occurrence of ESBL s synthesis among of these strains depends on clinical forms of nosocomial infections.

低能离子注入E.coli K12的HRS／IRR效应及recA基因在其诱发中的作用

以MG1655(野生型),LE392(recA-)和DH5α(recA-)3株E.coliK12菌株为材料,研究了30keVN+离子注入E.coliK12时HRS/IRR效应的诱发情况及recA基因在其诱发中的作用。结果显示:小于10×1014ions/cm2低剂量离子注入大肠杆菌可诱发HRS/IRR效应;30keVN+离子注入MG1655,LE392菌株都可诱发HRS/IRR效应,而在DH5α菌株中无法诱导IRR效应。recA-与HRS/IRR效应相斥性表明recA基因在HRS/IRR效应的诱发中发挥了重要作用。

指状青霉提取物诱发E.coli ND-160及K12 infA基因突变

背景与目的:研究指状青霉(Penicillium digitatum)提取物对大肠杆菌菌株的致突变性。材料与方法:采用E.coli ND-160菌株回复突变试验、K12infA基因突变试验及其突变序列分析。结果:指状青霉提取物:①可明显地诱导ND-160菌株回复突变;②对K12茼株可诱发其infA基因DNA序列中5个碱基位点突变,且其中1个位点的突变还可导致编码相应氨基酸的改变(Lys→val)。结论:指状青霉对大肠杆菌基因有明显的致突变性。

调控因子SlyA和RfaH在E.coli K4合成果糖软骨素中的生理作用

利用基因工程手段过量表达E.coli K4荚膜多糖(K4CPS)合成途径中相关代谢调控因子Sly A和Rfa H,以构建高效合成K4CPS的菌株。结果发现:sly A和rfa H基因的单独过量表达和共表达重组菌的K4CPS的产量较对照菌分别提高了81.8%、46.5%和153.8%;甘油比消耗速率较对照菌降低了12.5%、18.8%和31.3%,而乙酸含量则较对照菌降低了98.6%、39.7%和91.6%。因此,调控蛋白Sly A和Rfa H的过量表达能够大幅度提高E.coli K4的K4CPS合成,并增强菌体对甘油的利用率,而乙酸合成明显降低。而与单独表达策略相比,共表达策略能够更加有效地增强菌体合成K4CPS的能力。

用荧光抗体技术和肠细胞粘附试验检测K88^+E.coli对仔猪小肠上皮的粘附作用

细菌粘附到宿主粘膜表面是细菌致病的前提,在引起人、畜腹泻的大肠杆菌中已经发现了许多具有粘附作用的蛋白质抗原,例如 K88、K99、987P、F41、CFA/I、CFA/Ⅱ等抗原。这些抗原也叫菌毛或粘附素,它们位于菌体表面,能特异粘附到宿主小肠上皮细胞上,使细菌克服肠道蠕动的排斥在小肠内定居、繁殖。目前已经用遗传工程技术克隆3菌毛基因,用菌毛蛋白制成的疫苗,预防大肠杆菌腹泻,效果很好。在我国,新生仔猪大肠杆菌腹泻的发病率很高,仔猪腹泻大肠杆菌多数具有K88抗原,本实验建立了荧光抗体染色和肠细胞粘附二种方法,检测了K88+E.coli的粘附能力和菌毛的生物活性。

大肠杆菌MG1655菌株ERIC-PCR图谱主带序列组成分析

ERIC PCR已经在细菌分类、鉴定及混合菌群分析中得到广泛应用 ,但对其产物形成规律的认识仍存在分歧。以大肠杆菌MG1 655为对象 ,对其ERIC PCR指纹图谱中 1 1kb主带中的DNA片段进行了克隆、测序、基因组定位以及引物匹配分析。结果表明 ,这条1 1kb主带由分布在基因组中不同位置的 3种序列不同的片段组成 ,各片段的丰度差异较大 ,最高为 97 89% ;3种片段中的 2种所在的基因组区域仅一端含有ERIC序列。推测对含有ERIC序列的基因组DNA进行扩增时 ,ERIC PCR是一种非随机扩增。

19家医院大肠埃希菌和肺炎克雷伯菌中TEM型β-内酰胺酶的研究

目的检测全国19家医院大肠埃希菌和肺炎克雷伯菌中的TEM型ESBLs。方法收集2004～2005年全国19家医院对头孢他啶耐药的大肠埃希菌98株和肺炎克雷伯菌109株，琼脂稀释法测定菌株MICs，PCR扩增blaTEM基因。扩增阳性菌株进行接合实验，测定接合子MICs并PCR扩增blaTEM基因。扩增阳性的菌株和接合子以等电聚焦电泳（IEF）检测其β-内酰胺酶等电点。对具有典型TEM型ESBLs表型的菌株进行测序和变性高效液相色谱（DHPLC）分析。进一步收集检出突变菌株的宿主患者及其所在病房分离的对头孢他啶不敏感的菌株，进行测序、DHPLC分析，以及ERIC—PCR和RAPD分型。结果实验菌株中大肠埃希菌和肺炎克雷伯菌ESBL阳性率分别为84．7％和68．8％，blaTEM基因阳性率分别为67．3％和69．7％。仅1株大肠埃希茵P34表达TEM-12型ESBL，其他均为TEM-1（广谱β-内酰胺酶）。P34宿主患者分离的21株大肠埃希菌中有18株表达TEM-12，且所有菌株均为同一克隆。该患者住院期间所在病房分离的11株对头孢他啶不敏感大肠埃希菌均表达TEM-1，与P34均不是同一克隆，但不同患者间存在菌株的水平传播。结论TEM型ESBLs已在中国出现，但仍罕见，不是导致菌株对头孢他啶耐药的主要原因。本研究在国内首次报道了TEM-12型ESBL，该菌株虽未引起流行，但仍应引起重视。必须加强感染控制，防止TEM型ESBLs在中国的传播。

安徽地区PMQR基因阳性大肠埃希菌和肺炎克雷伯菌中ESBLs流行特征的研究

目的了解安徽地区临床分离含质粒介导的喹诺酮类耐药基因(PMQR)大肠埃希菌和肺炎克雷伯菌中编码超广谱β-内酰胺酶(ESBLs)的基因型别,及与PMQR基因在本地区共同传播的流行现状和耐药特征。方法采用琼脂稀释法测定40株临床分离含PMQR基因的大肠埃希菌与肺炎克雷伯菌对临床14种抗菌药物的药物敏感性,CLSI表型确证试验进行表型鉴定,PCR检测blaESBLs基因型;接合实验验证PMQR与blaESBLs基因的转移性;ERIC-PCR进行同源性分析。结果 40株PMQR阳性菌株对喹诺酮类药物显示耐药同时对多种β-内酰胺类药物耐药;PCR法检测PMQR阳性菌株中blaESBLs基因携带率达到60%(24/40),最常见的为CTX-M型ESBLs,检出率达到92%(22/24)。结论安徽地区临床存在PMQR与blaESBLs基因的共同传播及流行,包含PMQR基因的菌株多为产ESBLs菌株,同时携带PMQR与blaESBLs基因的菌株常为多药耐药菌。

产ESBLs大肠埃希菌和肺炎克雷伯菌的耐药性变化

目的分析产ESBLs大肠埃希菌和肺炎克雷伯菌的耐药性变化。方法收集我院2004年1月—2005年12月期间临床分离的大肠埃希菌和肺炎克雷伯菌,对其产ESBLs及耐药情况与2000年1月—2002年10月进行比较研究。结果以头孢噻肟为底物检测ESBLs,2004—2005年产ESBLs大肠埃希菌和肺炎克雷伯菌分别为35.4%和21.1%,与2000—2002年度比较显著增加(P<0.01)。2004—2005年产ESBLs大肠埃希菌和肺炎克雷伯菌占尿标本41.4%(133/321),呼吸道分泌物占29.0%(93/321),血液占5.9%(19/321),伤口分泌物占12.8%(41/321),体液或引流液占8.1%(26/321)。产ESBLs大肠埃希菌对氨曲南敏感性2004—2005年较前有显著下降(P<0.05),对其他抗生素的敏感性差异无统计学意义。产ESBLs肺炎克雷伯菌对抗菌药物的敏感性2004—2005年较2000—2002年除左氧氟沙星外均有下降趋势,并且头孢他啶、头孢哌酮-舒巴坦敏感性显著下降(P<0.05)。结论产ESBLs细菌近2年有增加趋势,并对多种抗生素的敏感性下降。

用CLSI和EUCAST两种标准判定产ESBLs菌株药敏结果的差异

目的分析美国CLSI标准和欧洲EUCAST标准判读产超广谱β-内酰胺酶(ESBLs)的大肠埃希菌(E.coli)和肺炎克雷伯菌(K.pneumoniae)对4种常用广谱头孢菌素药敏结果的差异。方法收集按CLSI标准因产ESBLs而将广谱头孢菌素药敏结果由敏感或中介改为耐药的E coli和K.pneumoniae,用琼脂稀释法检测最低抑菌浓度(MIC),用CLSI标准和EUCAST标准进行敏感性界定。同时用PCR及Hodge-test检测4种ESBLs基因和高活性β-内酰胺酶。结果55株菌中53株扩增出介导ESBLs的相关基因,Hodge-test显示55株菌均产高活性β-内酰胺酶;用EUCAST标准界定,55株菌株对头孢三嗪和头孢噻肟均耐药,对头孢他啶和头孢吡肟敏感的菌株分别有5和7株。结论在目前的耐药现状中,用CLSI规则和用EUCAST折点判读E.coli和K.pneumoniae对4种常用第三代和第四代头孢菌素敏感性,对临床治疗结果进行预测的差异主要出现在产ESBLs且头孢他啶和头孢吡肟MICs值≤1μg/m1的菌株中。

大肠杆菌K12碱性磷酸酶基因的克隆表达

大肠杆菌碱性磷酸酶是同二聚体金属酶,被phoA基因编码.采用PCR方法从大肠杆菌K12中扩增到碱性磷酸酶基因(phoA).用限制性内切酶BamHI和HindⅢ将片段插入克隆载体pETBlue-2.该基因被重组、转化后在大肠杆菌中经IPTG诱导表达,而后进行SDS-PAGE检测及紫外吸收分析测OD410.克隆得到了phoA基因并实现了蛋白表达,碱性磷酸酶的活性提高了18.3倍,为进行组织化学、免疫印迹、突变分析等工作打下了坚实的基础.

重组大肠埃希菌-厌氧梭菌穿梭质粒pIMP1-eIL-12稳定转化生孢梭菌

目的近些年来,以厌氧芽孢梭菌作为实体瘤基因治疗载体的研究逐渐受到关注。文中用重组人白细胞介素-12(rhIL-12)基因重组大肠埃希菌(E.coli)-厌氧梭菌穿梭质粒pIMP1,并稳定转化生孢梭菌,为增强杀伤肿瘤细胞的研究提供基础。方法用SOE-PCR法将rhIL-12基因连到厌氧梭菌的内源性β1,4-葡聚糖酶(endo-1,4-glucanase,eglA)启动子和信号肽之后,构建融合基因eglAp-rhIL-12,将其插入pIMP1,构建重组质粒pIMP1-eIL-12;重组质粒首先在E.coli DH5α内进行鉴定,然后用电穿孔法转化生孢梭菌;利用红霉素抗性筛选阳性克隆,并提取质粒鉴定阳性克隆。结果酶切和测序结果表明插入到pIMP1内的融合基因eglAp-rhIL-12序列及读框正确;抗生素压力筛选和20多代随机质粒提取酶切鉴定结果表明重组质粒pIMP1-eIL-12已稳定转化生孢梭菌。结论成功获得重组质粒pIMP1-eIL-12及其生孢梭菌稳定转化株,为以后的抗肿瘤研究奠定了基础。

噬菌体Bp7耐受株K12-R生物学特性分析

宿主菌E.coli K12的突变株K12-R不能被噬菌体Bp7裂解,为了明确其产生耐受的原因以及突变对其生物学性能的影响,对K12-R进行全基因组测序,分析其产生耐受的原因,浊度测定K12-R的生长曲线和自凝能力,革兰染色检测K12-R生物膜的形成能力,比较K12-R和E.coli K12之间生物学性能的变化。结果表明,突变株K12-R脂多糖合成相关基因hldE发生了突变,突变株K12-R细胞膜通透性增加,生长繁殖能力降低,自凝能力增强,生物膜形成能力增强。E.coli K12的脂多糖合成基因hldE突变能够改变K12-R脂多糖的结构,从而抑制噬菌体Bp7的吸附。这为明确K12-R突变株对噬菌体Bp7的耐受机制研究提供了理论依据。

Increasing Incidence of Extended-Spectrum Beta-Lactamase-Producing Enterobacteriaceae (ESBL) and the Relation to Consumption of Broad-Spectrum Antimicrobial Agents 2003-2011 in a Large Area of Copenhagen, Denmark

Purpose: To investigate 1) the development in the incidence of ESBL-producing bacteria in hospitals and primary health care, 2) the contribution of primary health care to the incidence of ESBL-producing bacteria, and 3) the development in resistance patterns for all Escherichia coli and Klebsiella pneumoniae isolates in relation to antimicrobial consumption in hospitals and primary health care. Methods: ESBL-data were retrospectively collected from bacterial isolates from all specimens received at the Department of Clinical Microbiology from 2003 to 2011 together with the corresponding patient data. ESBL-production was detected in isolates from 1067 of 59,373 patients (1.8%) with an E. coli infection and in 263 of 8660 patients (3.0%) with a K. pneumoniae infection. Results: From 2003 to 2009, an increase in patients with an ESBL-producing isolate occurred in both hospitals and primary health care at the same time as an increased consumption of broad-spectrum antimicrobial agents was seen. Interventions to reduce prescription of cephalosporins and ciprofloxacin at the hospitals from 2010 resulted in a remarkable decrease in patients with ESBL-producing K. pneumoniae whereas a continuing increase was seen in patients with ESBL-producing E. coli both at hospitals and in primary health care. The proportion of patients with community-acquired ESBL-producing E. coli was stable with an increase of only 1.4% from 2007 to 2011. Conclusions: Reduction in prescription of broad-spectrum antimicrobial agents at the hospital level had an important impact on the incidence of ESBL-producing K. pneumoniae, but not on ESBL-producing E. coli.

A novel mediator of the amyloid-βneurotoxicity in Alzheimerls disease:Ubiquitin conjugating enzyme E2-25K/Hip-2 as upstream of caspase-12

Accumulation of amyloid-β(Aβ) and its neurotoxicity are regarded as a major factor promoting neu-ronal degeneration in Alzheimer's disease (AD). Upon investigation of Aβtoxicity using DNA microarray, we isolated ubiquitin conjugating enzyme E2-25K/Hip-2 as a mediator of Aβ toxicity. Here we show that expression of E2-25K/Hip-2 was strongly up-regulated in the cultured cortical neurons exposed to Aβ1-42 in vitro and in vulnerable neurons surrounding senile plaques of the brain derived from AD patients and Tg2576 Alzheimer's mice. Aβ1-42-induced neurotoxicity, accumulation of ubiquitin conjugates, and decrease of the proteasome activity were mediated by ubiquitin ligase activity of E2-25K/Hip-2. Aβ-induced

MUC2基因表达对益生菌调节肠屏障作用的影响

目的观察益生菌诱导的乳鼠结肠MUC2基因的表达及其对益生菌抑制E.coli K1株E44黏附侵袭肠屏障作用的影响。方法 SD乳鼠分别用益生菌、E44株和益生菌+E44株三组灌胃7 d后,RT-PCR法观察益生菌和E44株诱导结肠MUC2基因的表达;靶向MUC2基因的shRNA真核质粒表达载体(shRNA MUC2)和阴性对照shRNA NC转染人结肠癌Lovo细胞,荧光定量PCR法检测其表达水平,并通过竞争性排斥方法检测MUC2基因对益生菌拮抗致病菌E44粘附侵袭的影响。结果灌胃益生菌组SD乳鼠肠道MUC2基因明显上调,而E44组则显著降低。用shRNA MUC2转染Lovo细胞后,与阴性对照组和空白对照组相比,其表达水平明显降低,干扰率为66.7%;益生菌对E44株粘附侵袭抑制作用明显低于未处理组,与对照组相比,E44相对粘附率为56.64%,相对侵袭率为66.64%。结论益生菌诱导的MUC2基因表达上调可能成为拮抗致病菌易位的保护机制之一;MUC2基因沉默后,益生菌对E44粘附侵袭肠上皮细胞的抑制作用明显降低。

家蚕抗菌肽CM4对大肠杆菌超微结构影响的研究(简报)

The effect of antibacterial peptide CM4 of Bombyx mori against E. coll K12 was investigated using scanning electron microscopy(SEM) and transmission electron microscopy (TEM). The ultrastructural changes of E. coli K12 were observed by the challenge of the purified antibacterial peptide CM4. The results showed that the antibacterial peptide caused a series of pathological changes on E. coli. SEM and TEM revealed aggregates of bacteria and SEM revealed wrin-kled bacterial surfaces in the early stage. Thereafter, plasmolysis was observed with irregular holes appearing in the two ends of bacteria and the cytoplasmic contents of the cells leaking out. Finally, bacteria became empty vesicles and disintegrated into small fragments subsequently. Comparatively, the bacterial membrane was normal and the bacterial structure remained intact in the control group.

黄粉虫幼虫免疫血淋巴最佳制样条件的确定

采用正交设计Ｌ２７（３１３）的方法对大肠杆菌诱导黄粉幼虫的免疫血淋巴最佳制样条件进行了研究，结果表明：以每虫１０５菌量诱导较小的虫体（０．７ｇ以下）后７２ｈ取样得到的样品活性最高。