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Tytuł pozycji:

Cellular locations of proteinases and association with vesicles in porphyromonas gingivalis

Tytuł:
Cellular locations of proteinases and association with vesicles in porphyromonas gingivalis
Autorzy:
Oishi S
Miyashita M
Kiso A
Kikuchi Y
Ueda O
Hirai K
Shibata Y
Fujimura S
Temat:
proteinase
enzyme
RGP
KGP
P. gingivalis
vesicle
Medicine
Źródło:
European Journal of Medical Research, Vol 15, Iss 9, p 397 (2010)
Wydawca:
BMC, 2010.
Rok publikacji:
2010
Kolekcja:
LCC:Medicine
Typ dokumentu:
article
Opis pliku:
electronic resource
Język:
English
ISSN:
2047-783X
Relacje:
http://www.eurjmedres.com/content/15/9/397; https://doaj.org/toc/2047-783X
DOI:
10.1186/2047-783X-15-9-397
Dostęp URL:
https://doaj.org/article/da4c635184d948708270ad023d76be05  Link otwiera się w nowym oknie
Numer akcesji:
edsdoj.4c635184d948708270ad023d76be05
Czasopismo naukowe
Abstract We found that locations of arginine-specific gingipain (RGP) in the cellular fractions in the crude extract, envelope, vesicles, and culture supernatants were 48%, 16%, 17%, and 31%, respectively, and the corresponding values of lysine-specific gingipain (KGP) were 47%, 10%, 7%, and 36%, respectively. Although the molecular mass of RGP in the culture supernatant had been determined as 43 kDa, and that of KGP had been as 48 kDa, molecular masses of both proteinases solubilized from the vesicles were estimated to be over 1,500 kDa, since they eluted in the void volume of the column in the gel filtration on Sephacryl S-300. There was no reduction of molecular size by the following treatment with SDS, high-concentration NaCl, or urea. Interestingly, the occurrence of the macromolecular forms could not observed in other enzymes tested such as monopeptidyl, dipeptidyl, and tripeptidyl peptidases, as well as alkaline phosphatase. Therefore, occurrence of the macromolecular forms may be restricted to the proteinases. When the vesicle and culture supernatants containing free RGP and KGP were mixed and incubated, neither RGP nor KGP seemed to bind to vesicles. RGP bound to the vesicle was found to be more stable to heat treatment than the free form, suggesting that association of RGP with the vesicle caused heat stability of this enzyme.

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