PROTEIN CAUSEING CELL AUTOAGGLUTINATION PROPERTY OF PLAGUE MICROBES, AND METHOD FOR PRODUCING IT

PROTEIN CAUSEING CELL AUTOAGGLUTINATION PROPERTY OF PLAGUE MICROBES, AND METHOD FOR PRODUCING IT

FIELD: medicine, pharmaceutics.SUBSTANCE: protein causing an Yersinia pestis cell autoagglutination property and located on a surface of the Yersinia pestis cell is recovered, and the presence thereof is correlated with an ability of bacteria to the autoagglutinaiton growth in liquid nutrient media...

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Bibliographische Detailangaben
Hauptverfasser: PODLADCHIKOVA OL'GA NIKOLAEVNA, RYKOVA VIOLETTA ANDREEVNA
Format: Patent
Sprache:eng ; rus
Schlagworte:
BEER
BIOCHEMISTRY
CHEMISTRY
ENZYMOLOGY
FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIREDCHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERSFROM A RACEMIC MIXTURE
METALLURGY
MICROBIOLOGY
MUTATION OR GENETIC ENGINEERING
ORGANIC CHEMISTRY
PEPTIDES
PROCESSES USING MICROORGANISMS
SPIRITS
VINEGAR
WINE
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Beschreibung
Zusammenfassung:FIELD: medicine, pharmaceutics.SUBSTANCE: protein causing an Yersinia pestis cell autoagglutination property and located on a surface of the Yersinia pestis cell is recovered, and the presence thereof is correlated with an ability of bacteria to the autoagglutinaiton growth in liquid nutrient media and with increased hydrophobic nature of the cells. Molecular weight of the protein makes 17.485 kDa, the protein content is 80%, and the neutral carbohydrate content is 6%. A method for producing the protein involves growing the strain of Y.pestis KM 1279 on 1.5% agar LB; the grown culture is washed off with cold buffered saline and dried with acetone. The cells are washed off and deposited by centrifugation in the cold; the cell deposition is suspended in NaOH (pH 9.0), kept in agitation at 26°C for two hours, and the cells are separated by centrifugation (8000 rpm). The supernatant is filtered through the membrane; the filtrate is added with neutralised ammonium sulphate to 25% saturation, kept to form a deposition to be separated by centrifugation and made free from ammonium sulphate by dialysis. The dialysed solution is added with HCl to pH 4.6, incubated to form a deposition, centrifuged; the deposition is dissolved in 5 mM NaOH. The protein is deposited by acetone, kept in the cold, centrifuged; and the deposition is lyophilised.EFFECT: protein is used for studying its protective properties, for creating on its basis vaccination preparations and assessing its involvement in realisation of the virulent properties of the plague agent.2 cl, 1 dwg, 2 tbl, 4 ex Выделен белок, обусловливающий свойство аутоагглютинации клеток Yersinia pestis, который расположен на поверхности клетки Yersinia pestis, и его наличие коррелирует со способностью бактерий к аутоагглютинативному росту в жидких питательных средах и с повышением гидрофобности клеток. Молекулярная масса белка 17,485 кДа, содержание белка 80%, углеводов нейтральных 6%. Способ получения белка включает выращивание штамма Y.pestis KM 1279 на 1,5% агаре LB, выросшую культуру смывают холодным забуференным физраствором и высушивают ацетоном. Клетки отмывают и осаждают центрифугированием на холоду, клеточный осадок суспендируют в растворе NaOH (pH 9,0), выдерживают при встряхивании при 26°С два часа и отделяют клетки центрифугированием (8000 об/мин). Супернатант фильтруют через мембрану, к фильтрату добавляют нейтрализованный раствор сульфата аммония до 25% насыщения, выдерживают до формирования осадка, который о