肉源隆德假单胞菌和致腐菌的混合生物被膜形成特征

为探究肉类优势腐败菌群的混合生物被膜互作规律,采用结晶紫法、苯酚硫酸法、二喹啉甲酸法和激光扫描共聚焦显微镜(CLSM)观察等分析在15℃和25℃肉源分离株隆德假单胞菌(PL)与3种致腐菌的混合生物被膜特性,及对蛋白酶和消毒剂耐受性的影响。结果表明,从腐败牛肉中分离鉴定的23株菌中,假单胞菌属占43.5%,其次为热杀索丝菌、不动杆菌属和类香味菌属。将优势腐败菌隆德假单胞菌与约翰逊不动杆菌、热杀索丝菌及类香味菌共培养,发现低温显著促进双菌混合生物被膜的形成。PL、AJ、BT在15℃时的生物被膜形成量均显著高于25℃时的,混合生物被膜在15℃时的形成量显著高于PL单培养的。PL与AJ共培养时,被膜菌数目比单培养时高0.75~0.78 lg(CFU/cm2),15℃共培养时,胞外多糖分泌量增加15.67~22.01μg/mL,与AJ、BT共培养的胞外蛋白分泌量分别增加7.35,6.70μg/mL。CLSM观察发现PL与MP或AJ混合生物被膜聚集团聚,形成不均一结构,被膜厚度增至48.99~49.22μm。此外,混合生物被膜的形成,显著提高假单胞菌的蛋白酶活性和化学耐受性。经0.06%次氯酸钠处理后,15℃时PL与AJ、BT混合被膜残留率高达95.61%,96.16%,显著高于PL单培养。结论:肉源致腐菌PL与3种致腐菌形成结构复杂的混合被膜,在低温环境下被膜菌增强对次氯酸钠的抵抗性,为探究肉源腐败微生物混合被膜的污染和控制奠定良好的基础。

基于法标的非洲地区水泥改良土基层路拌法快速施工技术

本文针对阿比让四桥工程的当地建设条件,确定水泥改良土基层路拌快速施工技术的核心及方案,通过实施试验段确定工艺流程、验收标准、施工参数及雨季控制措施,分析了项目应用效果及经济效益。

生鲜食品致腐假单胞菌生物被膜形成及其调控机制研究进展

假单胞菌是低温冷藏动物源性食品和果蔬的重要腐败菌,会造成食品品质劣变,从而导致严重的经济损失。致腐假单胞菌的致腐性与生物被膜形成密切相关,生物被膜能够增强该菌在食品加工和贮藏环境的生存和适应能力,引起持续和交叉污染。然而,与致腐相关的假单胞菌生物被膜形成及其机制仍缺乏系统的总结。本文介绍了生鲜食品中致腐假单胞菌的污染情况,分析了假单胞菌生物被膜形成及胞外基质的组成,重点阐述了致腐假单胞菌生物被膜形成的环鸟苷二磷酸、群体感应和小RNA分子等主要调控机制,为揭示生鲜食品来源的假单胞菌致腐机制及有效控制其生物被膜的污染提供理论参考。

加筋土拉拔试验的拉拔过程数值模拟

在土工布加筋黄土的拉拔试验基础上,建立FLAC3D数值分析模型,研究了拉拔试验中筋材拉应力、填土应力和位移的发展变化过程。研究表明:在拉拔过程中,筋材的拉应力随着拉拔位移增加而增大,当位移达到一定值后筋材拉应力保持不变;筋材拉应力沿筋长线性减小;筋土界面的交互作用会使得填土位移和应力重分布,拉拔端填料的水平土压力增大,而筋材末端填料的水平压力减小。填料的位移随拉拔位移增加而增大,且受影响的填料范围不断扩大,受影响区域填料的形状由椭圆形逐渐发展成水平放置的钟形。

Cell-free supernatants of Bacillus inhibit the biofilms of Pseudomonas lundensis cultured with and without Acinetobacter johnsonii

[Objective] Pseudomonas as one of the dominant spoilage bacteria highly form biofilms in chilled meat products and processing environment when contaminating single or mixed with other species.This study aims to investigate the antibiofilm properties of the cell-free supernatants(CFSs) of three Bacillus species isolated from fermented food and rice seeds on Pseudomonas lundensis(PL) or and Acinetobacter johnsonii(AJ) as mono-or dual-species.[Methods] Biofilm biomass,extracellular polymeric substances(EPSs),and biofilm structure were measured by crystal violet staining,spectrophotometry,confocal laser scanning microscopy(CLSM),respectively,as well as transcription of biofilm-related genes determined by qPCR.[Results] The CFSs of Bacillus amyloliquefaciens ZG08,B.velezensis B5,and B.subtilis YB11 inhibited the biofilm formation of PL and AJ without affecting their growth.The treatment with 50% CFSs of ZG08 and B5 decreased the cell viability of two biofilms by 12.73%–21.04%,which was higher than that of YB11(0.15%–4.38%).The inhibition rates of 50% CFSs of the three strains were 59.75%–79.59% against the PL biofilm and 63.62%–78.57% against the biofilm of PL+AJ,in which the CFS of YB11 had weaker activity.The content of exopolysaccharides and exoprotein in the two biofilms treated with these CFSs were reduced by 53.77%–73.30% and 54.84%–62.38%,respectively.The treatment with the three CFSs also reduced the adhesive cells,loosened biofilm structures,and thinned their thickness by 57.63%–74.49% and 60.43%–64.64%,respectively.Moreover,the CFSs of ZG08 and B5 effectively eradicated by 41.77%–69.79% against the mature biofilms of PL and PL+AJ,compared to weak activity of YB11.In addition,the antibiofilm activities of the three CFSs were stable under four enzyme digestion and heating conditions.Compared with the control,the CFSs of ZG08 and B5 significantly down-regulated the expression of six biofilm-related genes,lapA,alg44,pelG,luxR,wspR,and rpoS.[Conclusion] The CFSs of ZG08 and B5 have strong antibiofilm activities against PL and AJ as mono-or dual-species.

把牢企业基层党支部建设定盘星

基层党支部是党在基层社会中的前沿阵地和战斗堡垒,是党的活力的源泉和保障。随着社会经济的不断发展,作为基层党组织的企业党支部也需要在职能上不断与时俱进,满足时代对于其维护企业和谐稳定不断变化的要求,发挥其在促进企业稳定高效发展中的引领地位。把牢企业党支部建设＂定盘星＂,维护企业稳定发展。

双组分系统EnvZ/OmpR促进副溶血弧菌抵抗碱胁迫的作用机制

【目的】探究双组分系统(two-component system,TCS)EnvZ/OmpR对副溶血弧菌(Vibrio parahaemolyticus,VP)抵抗碱胁迫的作用机制。【方法】用SMART在线工具(https://smart.embl.de/)鉴定出副溶血弧菌基因组中的双组分系统EnvZ/OmpR,再利用同源重组技术将envZ和ompR基因分别进行缺失,构建相应回补株,比较各菌株的生长曲线来检测相应基因对细菌适应高渗透胁迫和碱胁迫的作用,并结合qRT-PCR及荧光检测系统,筛选参与EnvZ/OmpR抵抗碱胁迫的下游靶基因,鉴定该双组分系统对下游基因的调控机制。【结果】在副溶血弧菌基因组中鉴定出vp0155/vp0154编码EnvZ/OmpR双组分系统同源蛋白。ΔompR菌株在高渗透胁迫和碱胁迫中的生长能力明显弱于野生株,而回补株CΔompR、ΔenvZ和CΔenvZ菌株生长能力与野生株类似。在ΔompR菌株中,孔道蛋白基因vp1218、vp0493、vpa1745、vpa0085与vpa1308的转录水平均明显低于野生株,并且发现这些孔道蛋白基因缺失株(Δvpa1308除外)在碱性环境中生长能力均明显弱于野生株。OmpR蛋白可直接抑制调控因子AphB基因转录,而ΔaphB菌株在碱胁迫中的生长能力明显强于野生株。此外,AphB蛋白可直接抑制孔道蛋白基因vp0493和vpa0085转录。【结论】双组分系统EnvZ/OmpR促进副溶血弧菌抵抗碱胁迫,其中OmpR蛋白可通过抑制调控因子AphB的表达,以促进部分孔道蛋白的表达,从而增强副溶血弧菌抵抗碱胁迫的能力。