Vibrio cholerae O139 bacteriophages

Cholera bacteriophages have been isolated from 27 lysogenic cultures of V. cholerae O139. As shown the pages under study belong to two morphological groups A1 and F1 and serological types II and XII. The use of prophage typing and the sensitivity test to specific phage made it possible to differentiate V. cholerae strains, serogroup O139.     

Pili of a Vibrio cholerae O139

The pili of a strain of Vibrio cholerae O139 were purified and characterized. They were morphologically, electrophoretically and immunologically indistinguishable from the pili with 16 kDa subunit protein of V. cholerae O1. All 22 strains of V. cholerae O139 examined possessed the pili. The pili were different in hemagglutination inhibition pattern from V. cholerae O1 16K pili.     

Toxicity of Microcystis aeruginosa K-139 strain

Toxicity of the cells of a newly established axenic Microcystis aeruginosa K-139 strain to mice was studied. LD50 of the cells harvested in the mid-log phase was 7.3 mg/kg. The organs of acute dead mice were examined histopathologically. The blood congestion and necrosis of the parenchymal cells around the central veins in the liver were observed, but other organs seemed to be normal. The liver damage was confirmed by the tests of glutamic oxaloacetic transaminase (GOT) and glutamic pyruvic transaminase (GPT) activities in the sera of the mice after the injection with the K-139 cells. Furthermore, the K-139 cells were capable of inducing interleukin 1 (IL-1) production by peritoneal macrophages in vitro.     

Characterization of phage φ O139, a Vibrio cholerae O139 temperate bacteriophage with cohesive DNA termini

Abstract The cellular fatty acids and aldehydes of oral Eubacterium species were determined by gas chromatography-mass spectrometry. E. brachy and E. lentum contained mainly branched-chain fatty acids, whereas the others contained straight-chain acids. E. brachy E. lentum E. yurii ssp. yurii E. yurii ssp. margaretiae E. limosum E. plauti and E. aerofaciens also contained aldehydes with even carbon numbers. In addition to species-specific components, the compositional ratios of fatty acids and aldehydes characterized each individual species. The 10 species tested were divided into 5 groups by the principal component analysis. Cellular fatty acids and aldehydes would be chemical markers for interspecies differentiation of oral Eubacterium .     

Biosynthesis of the O Antigen from Citrobacter 139

The biosynthesis of the O antigen of Citrobacter 139 (Escherichia coli 3 Zurich 4,5,12:z(20)) was shown to proceed through a series of lipid-linked intermediates, similar to those involved in O-antigen synthesis in Salmonella. Galactose was the first sugar incorporated, followed by rhamnose and mannose. Abequose was incorporated from cytidine diphosphate (CDP)-abequose only when all three of the other nucleotide sugars (uridine diphosphate galactose, guanosine diphosphate mannose, and thymidine diphosphate rhamnose) were present. Rhamnosyl-galactosyl 1-phosphate and mannosyl-rhamnosyl-galactosyl 1-phosphate were identified as the products of mild alkaline hydrolysis of the lipid-linked intermediates.     

霍乱O139型菌苗的试制

对来自孟加拉、泰国、印度、中国四地区Ｏ１３９型霍乱菌株进行了毒力、免疫原性、免疫力与相互交叉保护力试验,结果显示不同地区分离的Ｏ１３９型霍乱弧菌其所试特性相互间无差异。用中国（９３－３）株试制的菌体菌苗,其抗原性、毒性、免疫力安全性等经检定符合霍乱菌苗规程要求。鉴于Ｏ１３９型霍乱弧菌存在荚膜的特性,而现有的几种荚膜多糖菌苗都显示有明显的保护作用,因而,使用Ｏ１３９型菌苗有可能在一定程度上达到控制Ｏ１３９型霍乱流行的目的。     

The role of residue S139 of mandelate racemase: synergistic effect of S139 and E317 on transition state stabilization

Mandelate racemase (MR) from Pseudomonas putida catalyzes the specific carbon-hydrogen bond cleavage of carbon acids with high pK (a) values. To further explore the catalytic mechanism of MR, "hot spots" contributing to transition state (TS) stabilization were identified by molecular dynamics (MD) simulations. MD simulations of MR with mandelic acid interpreted S139 in the active site cavity formed a hydrogen bond (HB) with one carboxyl oxygen of mandelate which also interacts with E317 through HB. Mutation of S139A by site-directed mutagenesis led to a significant reduction of catalytic efficiency ([Formula: see text]) about 45-fold and 60-fold in R?→?S and S?→?R directions, indicating the significance of Ser139 in mandelate racemization. MD of mutant S139A with mandelic acid efficiently provided insight for the decreased [Formula: see text] value and clearly demonstrated the synergistic effect of S139 and E317 on the stabilization of substrate at ground/TS.     

139 Development and application of crop exudate specific aptamers

The fertilizer industry is lucrative, though it faces environmental challenges. The amount of nitrogen applied to crops far exceeds the nitrogen utilized by crops leading to excess nitrogen in the form of nitrates, gaseous ammonia, and nitrogen oxides (DeRossa et al., 2010). This excess nitrogen can spread into groundwater contaminating drinking water and causing excess algal growth. Developments in nanotechnology may alleviate some of these environmental challenges. Although there are examples of nanotechnology being utilized for fertilizer products, none of these methods are able to respond to the specific nutrient needs of the plant. This project aims to produce a nanofertilizer product that can synchronize the release of its nutrients with the uptake of nutrients by the plant (DeRossa et al., 2010). Aptamers are synthetic molecules of DNA or RNA that can form 3-D shapes, which are capable of strongly and selectively binding a target of interest. Aptamers have been found to have binding affinities similar to, if not surpassing, those of monoclonal antibodies (Sultan et al., 2009). The goal of this project is to use polyelectrolyte microcapsules containing aptamers in their walls that are specific for key plant signals. This will allow the delivery of nutrient molecules from inside the microcapsules only when required by the plants. Root exudate specific aptamers are being developed using SELEX (Systematic Evolution of Ligands through Exponential enrichment) from a random DNA pool, as well as from an existing aptamer pool. These aptamers will act as molecular recognition probes in the development of an intelligent fertilizer system. Progress from these selections will be presented.     

Alkaline lipase production by Citrobacter freundii IIT-BT L139

Around 150 lipase producing bacterial isolates were screened from the local soils enriched with oil. Citrobacrer freundii IIT-BT L139, an isolated microbial strain, produced lipase that had high activity (8.8 U/ml) at pH 9.0 and 40 degrees C. The 16S rDNA phylogenetic studies showed that Citrobacter freundii belongs to the family Enterobacteriaceae and later confirmed by the microbial identification. Suitable C and N sources for lipase production were deduced to be starch and peptone-urea, respectively. In a controlled fermenter (1 L), the lipase activity was found to increase by 36% (12 Uml(-1)). The variation of lipase activity, pH and dissolved oxygen (DO) during growth of the organism in the controlled batch fermenter were monitored. The rheological characteristics of the fermentation broth indicated that it behaved like a Newtonian fluid throughout the fermentation. The fermentation time was comparatively short (60 h). The lipase was also found to be substantially resistant to common detergents. This lipase was, thus, characterized as alkaline, thermostable and solvent stable, which was essentially desirable in pharmaceutical, detergent and other industrial applications or production.     

Filamentous Phage fs1 of Vibrio cholerae O139

Filamentous phage, fs1, was obtained from Vibrio cholerae O139. The lysogenized strains produced a large amount of fs1 phage in the culture supernatant. This phage was previously reported as novel fimbriae of that organism. The genome of the phage was a 6.5 kb single-stranded DNA. The capsid of fs1 consists of a small molecule peptide (about 2.5 kDa).     

Lambdoid Coliphage HK139 Integrates Between his and supD

Phage HK139 is UV inducible and lambda homoimmune and has the host range of phi80. It can recombine with lambda as well as with phi80, and in the prophage form it is found integrated between the loci his and supD.