禽病原性大肠杆菌外膜蛋白的研究进展

大肠埃希氏富是家禽最常见的病原菌之一,可引起家禽胚胎死亡、脐炎、败血症、肉芽肿、卵黄性腹膜炎和全眼球炎等一系列疾病,给养禽业带来重大损失。禽病原性大O杆菌大部分属O1：K1、O2：K1和078：Kwlj以往国内外对禽源性大肠杆菌主要根据O抗原分型［1～3］。最近的研究结果显     

禽病原性大肠杆菌iro和tsh基因缺失株的构建

通过SSH和SCOTS研究, 铁系统(Iro)和温度敏感性血凝素(Tsh)在禽病原性大肠杆菌(APEC)的感染中可能发挥重要作用。基因检测发现, 在243个禽源大肠杆菌分离株中, 有205株为iro+菌株, 其中高、中度和低致病株分别为89.8%(184/205)、8.8%(18/205)和1.5%(3/205); 有167株为tsh+菌株, 高、中度、低致病株分别为87.4%(146/167)、12.6%(21/167)和0%(0/167), 结果显示iro+或tsh+株大多数为高致病株。为了确定iro和tsh基因在APEC致病力中的作用, 以APEC E037株为基础, 通过自杀性载体分别构建了iro和tsh基因缺失突变株E037(Δiro)、E037(Δtsh)和E037(ΔiroΔtsh)。动物感染性试验表明, 突变株在鸡体内的繁殖能力和致病性均明显下降, 但两个基因的协同致病作用不显著。进一步证实Iro和Tsh为APEC重要的致病因子。     

禽病原性大肠杆菌iro和tsh基因缺失株的构建

通过SSH和SCOTS研究, 铁系统(Iro)和温度敏感性血凝素(Tsh)在禽病原性大肠杆菌(APEC)的感染中可能发挥重要作用。基因检测发现, 在243个禽源大肠杆菌分离株中, 有205株为iro+菌株, 其中高、中度和低致病株分别为89.8%(184/205)、8.8%(18/205)和1.5%(3/205); 有167株为tsh+菌株, 高、中度、低致病株分别为87.4%(146/167)、12.6%(21/167)和0%(0/167), 结果显示iro+或tsh+株大多数为高致病株。为了确定iro和tsh基因在APEC致病力中的作用, 以APEC E037株为基础, 通过自杀性载体分别构建了iro和tsh基因缺失突变株E037(Δiro)、E037(Δtsh)和E037(ΔiroΔtsh)。动物感染性试验表明, 突变株在鸡体内的繁殖能力和致病性均明显下降, 但两个基因的协同致病作用不显著。进一步证实Iro和Tsh为APEC重要的致病因子。     

禽病原性大肠杆菌aes-31基因突变株的构建和致病性鉴定

【目的】通过禽病原性大肠杆菌(APEC)aes-31突变株的构建和动物实验来初步鉴定此基因片段对E058株的毒力影响。【方法】对在芯片杂交试验中筛选到的APEC E058株体外表达差异基因片段aes-31(来自SSH方法筛选到的E058株特异片段),用SSH引物从重组质粒中扩增出目的片段,克隆到pGEM-Teasy Vector中,然后用SphⅠ和SpeⅠ从中切下此片段,将之克隆到pMEG-375自杀性载体中,构建自杀性重组质粒pMEG375-aes-31,将突变载体转化到受体菌中,再和APEC E058株进行固相杂交,根据同源重组原理,筛选出基因突变株E058(Δaes-31)。【结果】E058株和突变株的LD50没有明显差别,突变株对35日龄SPF鸡的致死率高于E058株;两者接种鸡6 h内,E058(Δaes-31)突变株在各内脏器官和血液中的细菌数和E058株差异均不显著;接种鸡24 h后,E058(Δaes-31)突变株在脾脏和肺中的细菌数显著大于E058株,差异显著,E058(Δaes-31)突变株在心脏、肝脏和血液中细菌数显著大于E058株,差异极显著;接种鸡48 h后,E058(Δaes-31)突变株在心脏、肝脏和脾脏中的细菌数比E058株多,差异极显著,而肺脏和血液中的细菌数均无明显差异;48 h后突变株所引起的感染鸡的大肠杆菌病变比亲本株稍严重。【结论】以上数据表明aes-31有可能与E058株毒力的负调控有关。     

禽病原性大肠杆菌1型菌毛的分离与鉴定

以旋涡混合法使禽病原性大肠杆菌分离株566、1794和TK3菌毛脱落,经硫酸铵沉淀、透析后进行蔗糖密度梯度离心,收集密度为110至115g/cm3的蛋白带,经SDSPAGE测定,3株菌菌毛蛋白的分子量分别在175、170和170kD;提纯菌毛保留了甘露糖敏感性凝集豚鼠红细胞的能力,证明它们为1型菌毛;从1794株提取的1型菌毛免疫BALB/C小鼠产生的高免血清在Western blot中与3个菌株的相应菌毛蛋白均呈阳性反应。上述结果表明,受检的3株禽病原性大肠杆菌均表达了1型菌毛,其分子量在175～170kD之间,3个菌株的1型菌毛间具有较强的抗原相关性。     

江苏、安徽的禽致病性大肠杆菌

禽致病性大肠杆菌(Avian Pathogenic Escherichia coli,APEC)司引起禽类的多种疾病,是目前严重危害养禽业的传染病之一[1-2].APEC有复杂的血清型和广谱的耐药性,严重制约了该病的有效防控.最近的研究表明APEC能引起包括人在内的哺乳动物发病,提示APEC可能是人畜共患病的潜在病原体.因此,对APEC分子流行病学的研究,为进一步开展对该病的防控提供参考.     

大肠杆菌O121侵袭性菌株的发现与研究

本文报告从一急性腹泻患儿的脓血便中分离的具有侵袭性的大肠杆菌。该菌株发酵葡萄糖,产酸产气,不发酵乳糖,β-半乳糖苷酶试验阳性,在醋酸钠培养基上生长,赖氨酸脱羧酶阴性,无动力,能引起豚鼠角膜结膜炎,侵入上皮细胞,具有140Md的质粒带,经血清学试验证实其血清型为O121:H-,是国内外首次报道的新的侵袭性大肠杆菌血清型。     

大肠杆菌三型分泌系统2转录调节子EtrA对禽致病性大肠杆菌致病性的影响

【背景】禽致病性大肠杆菌(avian pathogenic Escherichia coli,APEC)是禽类主要病原菌之一,大肠杆菌三型分泌系统2 (Escherichia coli type III secretion system 2,ETT2)可通过转录调节子调控其致病性,但在APEC中转录调节子EtrA对其致病性的影响目前尚不清楚。【目的】研究ETT2中转录调节子EtrA对APEC致病性的影响。【方法】利用Red同源重组技术构建ETT2-etrA基因缺失株及回复株。比较生长性能、生物被膜形成、运动性及对血清敏感性的差异,基于RNA-Seq测序及Real-timePCR技术比较野生株和缺失株中与生物被膜形成、运动性以及毒力因子相关基因的转录水平。【结果】与野生株相比,缺失株及回复株生长特性无显著变化(P0.05),但APEC40-ΔetrA生物被膜形成能力和对血清敏感性明显增强(P0.001),运动性较野生株明显下降(P0.01),回复株的表型有所回复。转录组学筛选出7个毒力差异基因,生物被膜形成相关基因显著上调,参与影响细菌运动性的基因显著下调。qRT-PCR验证与转录组学结果一致。【结论】etrA缺失可以显著影响APEC的生物被膜形成、运动性及对血清的敏感性,这可为进一步探讨ETT2对APEC的致病作用提供参考。     

禽致病性大肠杆菌江苏、安徽分离株的生物学特性分析

[目的]研究禽致病性大肠杆菌(Avian Pathogenic Escherichia coli,APEC)江苏、安徽分离株的优势血清型,并分析其生物学特性.[方法]对分离自病禽的细菌进行鉴定,采用玻片凝集法测定禽致病性大肠杆菌的血清型,PCR方法检测14种毒力基因的分布,采用美国临床和实验室标准化研究所的方法进行药物敏感性检测,改良结晶紫半定量法检测分离细菌的生物被膜形成能力. [结果]共分离到禽致病性大肠杆菌56株,血清型检测结果表明,O78血清型占64.29％,为主要血清型.毒力基因检测显示,fimC、pfs、ompA和luxS的阳性率超过90％.药物敏感性检测显示,58.93％的菌株对8种以上的药物耐受.生物被膜检测显示,有16株细菌生物被膜形成能力为中等以上,其中68.75％的菌株耐8种以上的药物.[结论]O78为主要流行的血清型.fimC、pfs、ompA和luxS基因为APEC保守基因.多重耐药性仍很普遍,细菌生物被膜与耐药性具有相关性.     

我国部分地区禽源性大肠杆菌的外膜蛋白型

测定了从我国１８个省、市、自治区分离到的２０４个禽病原性大肠杆菌优势血清型分离株的外膜蛋白型（ＯｕｔｅｒＭｅｍｂｒａｎｅＰｒｏｔｅｉｎＰａｔｅｒｎｓ,ＯＭＰ型）。这些分离株共产生了４个ＯＭＰ型,５６个Ｏ１８分离株可分为３个ＯＭＰ型,５４个Ｏ７８分离株、２８个Ｏ２分离株、２６个Ｏ８８分离株、２２个Ｏ１１分离株和１８个Ｏ２６分离株,分别出现了４、２、１、３和１个ＯＭＰ型。其中,ＯＭＰ１型为６个血清型所共有,ＯＭＰ３型则同时存在于Ｏ１８、Ｏ７８、Ｏ２和Ｏ１１分离株中。结果表明,优势血清型中,Ｏ１８、Ｏ７８、Ｏ２和Ｏ１１分离株具有多样性的ＯＭＰ型,而Ｏ８８、Ｏ２６分离株的ＯＭＰ型则高度一致,所测６个优势血清型的分离株间存在共同的ＯＭＰ型     

Identification of genes transcribed by Haemophilus parasuis in necrotic porcine lung through the selective capture of transcribed sequences (SCOTS)

Haemophilus parasuis is the aetiological agent of Glässer's disease, which has received more attention in the past decade due to the increasing economic losses in the pig industry worldwide. Little is known about the mechanisms by which H. parasuis survives in the host. In this study, selective capture of transcribed sequences (SCOTS) was used to identify H. parasuis genes upregulated in necrotic porcine lung 7 days post infection. Thirty‐eight genes were identified that were upregulated during infection of the lung tissue of pigs, compared with growth in culture medium. In two examples chosen gene expression was not confined to the lungs, there being variation between tissues. The data support biofilm formation being an important mode of growth for colonization and/or persistence. Results from the in vitro studies suggest that, as for other pathogens, iron and oxygen restriction and heat stress are important environmental signals to regulate gene expression. This study has identified genes of H. parasuis that are upregulated during infection of porcine lung tissue as compared with in vitro growth conditions.     

Use of selective capture of transcribed sequences to identify genes preferentially expressed by Streptococcus suis upon interaction with porcine brain microvascular endothelial cells

By using the selective capture of transcribed sequences (SCOTS) approach, we identified 28 genes preferentially expressed by the major swine pathogen and zoonotic agent Streptococcus suis upon interaction with porcine brain microvascular endothelial cells. Several of these genes may be considered new S. suis candidate virulence factors. Results from this study demonstrate the suitability of SCOTS for the elucidation of gene expression in streptococcal species and may contribute to a better understanding of the pathogenesis of S. suis infections.     

23种中草药体外抗菌活性筛选

为研究23种中草药的80%乙醇提取物对4种临床常见致病菌的体外抗菌活性,该研究用琼脂扩散法测定抑菌圈直径,微量肉汤培养基倍比稀释法测定最低抑菌浓度(minimum inhibitory concentration,MIC)和最低杀菌浓度(minimum bactericidal/fungicidal concentration,MBC/MFC)。结果表明:滇龙胆草、金丝梅、溪黄草等16种提取物对金黄色葡萄球菌的MIC/MBC值在0.19～3.12 mg·mL^-1之间,有很强的抑菌活性。头花蓼、淡竹叶、半枝莲等14种提取物对铜绿假单胞菌的MIC/MBC值在1.56～6.25 mg·mL(-1)之间,有较强的抑菌活性。除槐角外,其余提取物对大肠埃希菌的MIC/MBC值均在3.12～12.5 mg·mL^-1之间,有较强的抑菌活性。黄藤、藿香提取物对白色念珠菌的MIC/MFC值在0.78～6.25 mg·mL^-1之间,有较强的抑菌活性;滇龙胆草、金丝梅、水杨梅、苦参、胡椒、赶黄草、荜菝、淡竹叶提取物对白色念珠菌的MIC/MFC值...     

Similar tissue-specific expression of the Adh genes from different Drosophila species is mediated by distinct arrangements of cis-acting sequences

In Drosophila melanogaster transformants, the alcohol dehydrogenase (Adh) genes from D. affinidisjuncta and D. grimshawi show similar levels of expression except in the adult midgut where the D. affinidisjuncta gene is expressed about 10- to 20-fold more strongly. To study the arrangement of cis-acting sequences responsible for this regulatory difference, homologous restriction sites were used to create a series of chimeric genes that switched fragments from the 5 and 3 flanking regions of these two genes. Chimeric genes were introduced into the germ-line of D. melanogaster, and Adh gene expression was analyzed by measuring RNA levels. Various gene fragments in the promoter region and elsewhere influence expression in the adult midgut and in whole larvae and adults. Comparison of these results with earlier studies involving chimeras between the D. affinidisjuncta and D. hawaiiensis genes indicates that expression in the adult midgut is influenced by multiple regulatory sequences and that distinct arrangements of regulatory sequences can result in similar levels of expression both in the adult midgut and in the whole organism.     

Biocatalytic synthesis of monocyclic arene-dihydrodiols and -diols by Escherichia coli cells expressing hybrid toluene/biphenyl dioxygenase and dihydrodiol dehydrogenase genes

The hybrid toluene/biphenyl dioxygenase, which is encoded by the todC1 gene of Pseudomonas putida F1 and the bphA2A3A4 genes of Pseudomonas pseudoalcaligenes KF707, has substrate ranges wider than toluene dioxygenase endoced by the todC1C2BA genes of P. putida F1. We carried out growing cell reactions by Escherichia coli expressing the todC1-bphA2A3A4 genes for the comprehensive production of monocyclic arene-dihydrodiols. As a result, we successfully biotranformed acetophenone-related compounds (acetophenone, propiophenone, and butyrophenone) to the corresponding cis-dihydrodiols. Furthermore, we performed the bioconversion experiments by E. coli cells expressing the bphB (dihydrodiol dehydrogenase) gene in addition to todC1-bphA2A3A4 to produce a series of monocyclic arene-diols. Consequently, toluene, benzene, stylene, p-xylene, acetophenone, propiophenone, butyrophenone, and trifluoroacetophenone were converted to the corresponding vicinal diols. The antioxidative activity of these generated diol compounds was markedly higher than that of the substrate used.     

从烟草EST微卫星标记中筛选合子胚中优势表达的基因

为获得烟草合子胚中的优势表达基因,利用CAP3程序对来自烟草公共数据库的EST序列进行组装,利用MISA程序从组装后的EST中筛选SSR位点,将多态性的SSR位点在烟草合子文库中进行扩增并对等位基因进行分析。结果表明:具有多态性的16个SSR标记中,有9个基因能从烟草的合子库中成功扩增得到。该研究为筛选烟草合子胚中优势表达基因提供新的途径。     

Somatic homologous recombination in planta: The recombination frequency is dependent on the allelic state of recombining sequences and may be influenced by genomic position effects

The Escherichia coli sodA gene encoding the antioxidant enzyme Mn-containing superoxide dismutase (MnSOD), was cloned in the expression vector pMG36e. This vector has a multiple cloning site down-stream of a promoter and Shine-Dalgarno sequences derived from Lactococcus. The protein-coding region of sodA from E. coli was amplified by the polymerase chain reaction, using a thermocycler and Taq DNA polymerase before cloning into pMG36e. When introduced into E. coli, the recombinant plasmid expressed the predicted fusion protein, both in the presence and absence of oxygen. The expression of the fusion protein in E. coli was verified by SOD assays, activity gels and Western blots. The recombinant plasmid was also introduced into Lactococcus lactis, which contains a resident SOD, and into Lactobacillus gasseri, which is devoid of SOD. Transformed lactococci expressed an active SodA fusion protein plus an active hybrid protein composed of subunits of the Lactococcus and the recombinant E. coli enzymes. Transformants of L. gasseri expressed only the fusion SodA protein, which was enzymatically active.