Amplified expression, purification and functional reconstitution of the dipeptide and tripeptide transport protein of Lactococcus lactis

Hagting, A.; Knol, J.; Hasemeier, B.; Streutker, M.R.; Fang, G.; Poolman, B.; Konings, W.N.

Amplified expression, purification and functional reconstitution of the dipeptide and tripeptide transport protein of Lactococcus lactis

1997

Transport of hydrophilic dipeptides and tripeptides into Lactococcus lactis is mediated by a proton-motive-force-driven peptide-transport protein (DtpT) that shares similarity to eukaryotic peptide trans-porters, e.g. from yeasts, plants, and the kidney and small intestine of rabbit, man and rat. The expression level of DtpT protein in L. lactis was increased (20-40-fold) to approximately 10% of total integral membrane protein by means of a low-copy-number vector and selecting the appropriate growth conditions. Membrane vesicles bearing the DtpT-His6 protein (containing a C-terminal factor-Xa cleavage site and a six-histidine-tag) showed a Pro-Ala uptake activity that was half that of membranes containing the wild-type protein. The activity in the DtpT-His6 membrane vesicles increased at least 50% upon removal of the His6 tag from the protein. More than 95% DtpT was solubilized from L. lactis membranes in the presence of 1% (mass/vol.) n-dolecyl-beta-n-maltoside, and approximately 2 mg DtpT-His6 was purified by Ni2+ -chelate affinity chromatography from 100 mg membrane protein. Purified DtpT-His6 was reconstituted unidirectionally into detergent-saturated formed liposomes, which were prepared from Escherichia coli phospholipid and egg phosphatidylcholine; the detergent was removed by adsorption to polystyrene beads. The highest uptake activities were obtained when DtpT was incorporated into liposomes that were treated with a low amount of n-dodecyl-beta-D-maltoside (onset of liposome solubilization). The uptake activity could be improved by addition of NaCl (200 millimole) and lipids (2 mg/ml) during the solubilization, purification and reconstitution steps.

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Ключевые слова АГРОВОК

adsorption animals bacterial proteins biosynthesis carrier proteins cloning dipeptides dipeptides eggs escherichia coli humans hydrophilicity intestine kidneys kinetics lactococcus lactis metabolism mutagenesis nickel oligopeptides phosphatidylcholines plants rabbits rabbits rats rats recombinant proteins saccharomyces cerevisiae small intestine sodium chloride solubilization transport proteins yeasts

Библиографическая информация

Опубликовано в

European journal of biochemistry

Том 247 Выпуск 2 Нумерация страниц 581 - 587 ISSN 0014-2956

Издатель

American Chemical Society, Books and Journals Division]

Другие темы

Molecular; Membrane transport proteins; Tripeptides; Isolation & purification; Affinity chromatography; Site-directed; Kidney; Polystyrenes; Sequence tagged sites; Small

Язык

Английский

Тип

Journal Article; Text

В АГРИСе с: 2024-02-27

Формат: MODS

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Эту запись предоставил National Agricultural Library

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Ссылки

DOI DOI http://dx.doi.org/10.1111/j.1432-1033.1997.00581.x

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Amplified expression, purification and functional reconstitution of the dipeptide and tripeptide transport protein of Lactococcus lactis

1997

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Библиографическая информация