The outer membrane of Proteus mirabilis. II. The extractable lipid fraction and electron-paramagnetic resonance analysis of the outer and cytoplasmic membranes.

1. The lipid fraction extracted from the outer and cytoplasmic membranes of Proteus mirabilis with chloroform/methanol consisted almost entirely of phosphatidylethanolamine, diphosphatidylglycerol and phosphatidylglycerol. 2. The phospholipid content of the cytoplasmic membrane was more than twice that of the outer membrane (38% as against 18% of the total dry weight) and the proportions of the three phospholipids differed somewhat in the two membranes. Yet, the fatty acid composition of the extractable lipids was essentially the same in both membranes. 3. The freedom of motion of spin-labeled fatty acids in the outer membrane of P. mirabilis depended markedly on temperature and on the position of the nitroxide group on the hydrocarbon chain of the probe, suggesting that the local environment of the probe is an associate lipid structure with the properties of a bilayer. Nevertheless, the mobility of the probe was more restricted in the outer membrane than in the cytoplasmic membrane, indicating a higher viscosity of the outer membrane. 4. Chloroform/methanol completely removed the phospholipids from the outer membrane, leaving the lipopolysaccharide moiety intact. The motion of spin-labeled fatty acids in the extracted membranes was, however, highly restricted, suggesting that, in the native outer membrane, the local environment of the probe is composed of phospholipids rather than lipopolysaccharide. Aqueous acetone extraction removed only 75-80% of the phospholipids of the outer membrane. Nevertheless, the mobility of the spin-labeled fatty acid remained highly restricted, suggesting the existence of two phospholipid environments in the outer membrane differing in the nature of their association with the lipopolysaccharide and protein moieties.     

Interspecies recA protein substitution in Escherichia coli and Proteus mirabilis

Summary With the help of recombinant plasmids carrying the recA gene of Escherichia coli or of Proteus mirabilis the ability of the recA gene products to substitute functionally for each other was studied. The recA protein of each can function in recombination, repair, induction of mutations and prophages and in regulation of its own synthesis within the foreign host nearly equally well as in the natural host. It is, therefore, suggested that recA-dependent processes act similarly in E. coli and P. mirabilis.     

Effect of the Proteolytic Enzymes of Bacillus licheniformis and the Lysoamidase of Lysobacter sp. XL1 on Proteus vulgaris and Proteus mirabilis Cells

Preparations of culture liquid of three Bacullus licheniformis strains (S, 103, and 60.4) and the enzymatic preparation lysoamidase from culture liquid of Lysobacter sp. strain XL1 actively lysed pre-autoclaved cells of the gram-negative bacteria Proteus vulgaris and P. mirabilis. Living Proteus cells treated with these enzymatic preparations were lysed during their subsequent autoclaving. Inoculation of enzyme-treated Proteus cells, taken either separately or in combination with one another and polymyxin B, into a rich medium led to cell repair and restoration of the culture viability. __________ Translated from Prikladnaya Biokhimiya i Mikrobiologiya, Vol. 41, No. 5, 2005, pp. 558–563. Original Russian Text Copyright ? 2005 by Ryazanova, Ledova, Tsurikova, Stepnaya, Sinitsyn, Kulaev.     

Swarming Characteristics of Proteus mirabilis Under Anaerobic and Aerobic Conditions

Nutrients have a pronounced effect on the growth and swarming behaviour of Proteus mirabilis 7002. Iron, zinc, amino acids, and dioxygen are important for rapid growth and normal swarming. Anaerobically grown cultures of P. mirabilis 7002 were unable to swarm on anaerobically maintained rich nutrient agar. Upon exposure to aerobic conditions, P. mirabilis 7002 resumed swarming behaviour. Scanning electron microscopy was used to demonstrate the presence of community organization and mature rafts during normal swarming. These results support the importance of dioxygen and redox status in cell differentiation.     

Heterologous Expression and Characterization of L-Amino Acid Deaminase from Proteus mirabilis in Escherichia coli

We expressed an L-amino acid deaminase (Pma) from Proteus mirabilis (P. mirabilis) in Escherichia coli and characterized the kinetics of phenylpyruvic acid production. P. mirabilis Pma was well expressed in E. coli in an active state and was found to be associated with membranes. The association of Pma with cellular membranes is likely to be necessary for its enzymatic activity.     

鸡源奇异变形杆菌分离鉴定及生物学特性

【背景】奇异变形杆菌(Proteusmirabilis,PM)是人畜共患病原菌,在自然界分布广泛。近年来,随着畜禽奇异变形杆菌病发病率上升和耐药性增强,亟需开展对该菌的防控研究。【目的】分离鉴定鸡源奇异变形杆菌,鉴定其耐药性、致病性、生物被膜形成能力等生物学特性。【方法】采用聚合酶链式反应(Polymerase Chain Reaction,PCR)方法鉴定了从2019-2020年病鸡中分离的52株临床奇异变形杆菌。分别采用药敏试验、PCR、结晶紫染色法对临床菌株的耐药性、毒力基因及生物膜的形成进行研究。【结果】选择14株代表性菌株进行16SrRNA基因测序,结果表明所测分离菌株均为奇异变形杆菌。所有分离菌株均对克林霉素、阿奇霉素、红霉素、四环素和利福平耐药,对氯霉素和头孢曲松外的抗生素耐药性均高于50%。对分离的奇异变形杆菌的13个毒力基因检测表明,所有菌株均能检测到hpmA、hpmB、rpoA、mrpA、fliL、zapA、ureC、atfC、atfA、pmfA,而ucaA和rsbA检出率分别为19.23%(10/52)和48.08%(25/52),hlyA未检出。对分离株生物被膜形成能力检测结果表明,所有菌株均能形成生物被膜,19.23%(10/52)的分离菌株形成生物被膜能力强,而且25℃条件下成膜能力比37℃更强。【结论】鸡源奇异变形杆菌携带多种毒力基因,具有较强生物被膜形成能力,耐药模式多样且日趋严重,应进一步加强对奇异变形杆菌在动物致病性和耐药性方面的监控,以降低其感染风险。     

Biochemical characterization of a novel lysine racemase from Proteus mirabilis BCRC10725

A lysine racemase gene (lyr) that consisted of an open reading frame of 1224-bp and encoded a protein with a calculated molecular mass of 45 kDa was cloned from the Proteus mirabilis BCRC10725 and expressed in Escherichia coli BL21(DE3). The purified His₆-tagged Lyr was most active towards lysine, exhibiting a specific activity of 2828 ± 97 U/mg. This enzyme also racemized arginine with a specific activity of 568 ± 28 U/mg but not other amino acids. The optimal conditions for Lyr activity to l-lysine were pH 8.0–9.0 and 50 °C. The racemization activity of Lyr was completely inhibited by 5 mM hydroxylamine and was partially restored by the addition of pyridoxal 5′-phosphate. The S394 residue of Lyr was subjected to site-directed mutagenesis. The arginine racemization activities of the S394Y, S394N, S394C and S394T variant proteins were increased by 1.5–1.8 fold compared to the wild-type Lyr, indicating that the S394 residue played a crucial role in determining the preference of Lyr to lysine and arginine.     

长春地区鸡源奇异变形杆菌的分离鉴定及毒力分析

【背景】奇异变形杆菌(Proteus mirabilis)是一种机会致病菌,广泛存在于周围环境中,常导致动物和人类感染。【目的】探究吉林省长春地区某养鸡场病鸡死亡原因,为疾病防控提供参考。【方法】从病死青年鸡脏器分离到病原菌TSA-1,通过革兰氏染色、生化试验和16S rRNA基因序列鉴定,并进行药敏试验、毒力基因检测、细胞毒性和黏附性试验、大蜡螟攻毒试验研究。【结果】分离株TSA-1在镜下呈短杆状、球状的革兰氏阴性菌,生化特性与奇异变形杆菌相一致,16S rRNA基因序列比对显示与奇异变形杆菌相似度为100%;药敏试验结果显示分离株TSA-1对氨苄西林、四环素、卡那霉素、头孢唑林等14种药物耐药,对环丙沙星、恩诺沙星等7种药物敏感;分离株还具有较强的生物被膜形成能力,携带ireA、ucaA、pmfA、atfA、ptA、zapA、hpmA和flhC这8种毒力基因,并对巨噬细胞RAW264.7表现出细胞毒性,而且对Caco-2细胞具有很强的黏附作用;同时对大蜡螟幼虫表现出比禽致病性大肠杆菌(avian pathogenic Escherichia coliO78,APEC-O78)更强的致死作用。【结论】从病死鸡脏器分离得到的奇异变形杆菌TSA-1具有多重耐药性,并携带多种毒力基因,对细胞和大蜡螟幼虫表现出强毒性作用,说明该菌是引起病鸡死亡的主要致病菌之一,应引起重视。     

Functional substitution of the recE gene of Bacillus subtilis by the recA gene of Proteus mirabilis

Summary Rec mutants of Bacillus subtilis have been tested for complementation by the recA gene of Proteus mirabilis (recApm) which was introduced into B. subtilis via the plasmid pHP334. In the recE4 mutant of B. subtilis the plasmid pHP334 restored significantly the defects in RecE functions tested: UV-sensitivity, homologous recombination (transduction and transformation) and prophage induction.Although serological methods to detect the presence of RecApm protein in B. subtilis have been unsuccessful, our results strongly indicate that the recE function of B. subtilis is analogous to the recA function of P. mirabilis.Abbreviations Cm^r resistance to chloramphenicol - Em^r resistance to erythromycin - Tc^r resistance to tetracycline - SDS sodium dodecyl sulfate - UV ultraviolet - AS ammonium sulfate     

基于多重计算设计策略提高奇异变形杆菌脂肪酶的热稳定性

来自奇异变形杆菌的脂肪酶(Proteus mirabilis lipase,PML)具有较好的有机溶剂耐受性,在生产生物柴油等领域有广泛的应用潜力.然而,其热稳定性仍有待提高以更好地适应工业生产.近年来,基于计算机辅助的多种计算设计策略的发展为酶的热稳定性改造提供了更多的思路.文中首先选择了 3种基于互补算法的软件AB...     

Comprehensive inhibitor profiling of the Proteus mirabilis metalloprotease virulence factor ZapA (mirabilysin)

In this study we report for the first time the comprehensive inhibitor profiling of the Proteus mirabilis metalloprotease virulence factor ZapA (mirabilysin) using a 160 compound focused library of N-alpha mercaptoamide dipeptides, in order to map the and binding site preferences of this important enzyme. This study has revealed a preference for the aromatic residues tyrosine and tryptophan in and aliphatic residues in . From this library, six compounds were identified which exhibited sub- to low-micromolar K_i values. The most potent inactivator, SH–CO₂–Y–V–NH₂ was capable of preventing ZapA-mediated hydrolysis of heat-denatured IgA, indicating that these inhibitors may be capable of protecting host proteins against ZapA during colonisation and infection.     

Study of the cytoplasmic and outer membranes of Escherichia coli by deuterium magnetic resonance.

The cytoplasmic and outer membranes of Escherichia coli were studied between 0 and 40 degrees C by deuterium magnetic resonance quadrupolar echo spectroscopy. The L51 strain of E. coli was used to incorporate perdeuterated palmitic acid into the membrane phospholipids. The cytoplasmic and outer membranes were separated using standard techniques. The spectrum of each membrane preparation was dominated at high temperatures (greater than or equal to 37 degrees C) by the characteristic liquid-crystalline plateau previously observed for perdeuterated palmitate chains in model phospholipid membranes. At low temperatures, the shape and width of the spectrum were characteristic of the gel phase. The relative intensities of the liquid-crystalline and gel features varied systematically with temperature. A quantitative analysis of the acyl chain orientational order was carried out by using the method of moments. The orientational order at each temperature was greater in the outer membrane sample than in that of the cytoplasmic membrane, indicating that the liquid-crystalline-gel transition region in the outer membrane is shifted to higher temperatures than that of the cytoplasmic membrane by about 7 degrees C. It is clear from the results that most of the phospholipid molecules participate in the phase transition.     

Translocation of an outer membrane protein into prey cytoplasmic membranes by bdellovibrios.

Within minutes of Bdellovibrio bacteriovorus attack on prey cells, such as Escherichia coli, the cytoplasmic membrane of the prey is altered. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of purified invaded prey cell (bdelloplast) membranes revealed the appearance of a noncytoplasmic membrane protein. This protein is not observed in preparations of noninvaded E. coli membranes and migrates in a manner similar to that of E. coli OmpF. Isoelectric focusing and two-dimensional gel electrophoresis of bdelloplast cytoplasmic membrane preparations also revealed the presence of a protein with electrophoretic properties similar to those of OmpF and the major Bdellovibrio outer membrane proteins. The protein appears in cytoplasmic membrane preparations within minutes of attack and persists throughout most of the intraperiplasmic developmental cycle. The appearance of this protein is consistent with our hypothesis that bdellovibrios translocate a pore protein into the bdelloplast cytoplasmic membrane to kill their prey and to gain access to the cytoplasmic contents for growth.     

碱性羟胺、弱碱和乙酸水解奇异变形杆菌LPS抗原及其活性的影响

采用碱性羟胺、弱碱、乙酸水解奇异变形杆菌LPS抗原,研究不同方式对小鼠活性的影响。检测结果表明,与水解前对比三种方式均能降低LPS抗原内毒素含量,即从2 500×104EU/mL降低至(250~2.5)×104EU/mL;热源性检测表明对家兔体温几乎无影响;但免疫原性结果表明ED50 LPSED50 Acid-LPS+Al(OH)3ED50 Alkaline-LPS+Al(OH)ED350 HA-LPS+Al(OH),3毒性结果为LD50 HA-LPSLD50 Alkaline-LPSLD50 LPSLD50 Acid-LPS。因此,经过乙酸(体积分数2%)或0.1 mol/L弱碱(体积分数2%)水解,能够显著降低内毒素含量及热源性,并保持其生物活性,使之成为有效的候选疫苗组分,用于预防或治疗大面积烧伤及术前或术后感染。     

Cytoplasmic membrane vesicles of Escherichia coli. A simple method for preparing the cytoplasmic and outer membranes.

A simple preparative method is described for isolation of the cytoplasmic and outer membranes from E. coli. The characteristics of both membrane fractions were studied chemically, biologically, and morphologically. Spheroplasts of E. coli K-12 strain W3092, prepared by treating cells with EDTA-lysozyme [EC 3.2.1.17], were disrupted in a French press. The crude membrane fraction was washed with 3 mM EDTA-10% (w/v) sucrose, pH 7.2, and the cytoplasmic membranes and outer membranes were separated by sucrose isopycnic density gradient centrifugation. The crude membrane fraction contained approximately 10% of the protein of the whole cells, 0.3% of the DNA, 0.7% of the RNA, 0.3% of the peptidoglycan, and about 30% of the lipopolysaccharide. The cytoplasmic membrane fraction was rich in phospholipid, while the outer membrane fraction contained much lipopolysaccharide and carbohydrate; the relative contents of lipopolysaccharide and carbohydrate per mg protein in the cytoplasmic membrane fraction were 12 and 40%, respectively, of the contents in the outer membrane fraction. Cytochrome b1, NADH oxidase, D-lactate dehydrogenase [EC 1.1.1.28], succinate dehydrogenase [EC 1.3.99.1], ATPase [EC 3.5.1.3], and activity for concentrative uptake of proline were found to be localized mainly in the cytoplasmic membranes; their specific activities in the outer membrane fraction were 1.5 to 3% of those in the cytoplasmic membrane fraction. In contrast, a phospholipase A appeared to be localized mainly in the outer membranes and its specific activity in the cytoplasmic membrane fraction was only 5% of that in the outer membrane fraction. The cytoplasmic and outer membrane fractions both appeared homogeneous in size and shape and show vesicular structures by electron microscopy. The advantages of this method for large scale preparation of the cytoplasmic and outer membrane fractions are discussed.