CHARACTERIZATION OF AN AMYLASE-BINDING COMPONENT OF STREPTOCOCCUS-GORDONII-G9B

被引：30

作者：

SCANNAPIECO, FA ^{[1
]}

HARASZTHY, GG ^{[1
]}

CHO, MI ^{[1
]}

LEVINE, MJ ^{[1
]}

机构：

[1] SUNY BUFFALO,SCH DENT MED,DENT RES INST,BUFFALO,NY 14214

来源：

INFECTION AND IMMUNITY | 1992年 / 60卷 / 11期

关键词：

D O I：

10.1128/IAI.60.11.4726-4733.1992

中图分类号：

R392 [医学免疫学]; Q939.91 [免疫学];

学科分类号：

100102 ;

摘要：

The goal of the present study was to begin characterizing the amylase-binding component(s) on the surface of Streptococcus gordonii G9B. Alkali extracts but not phenol-water extracts of this bacterium inhibited I-125-amylase binding to S. gordonii G9B. To identify the bacterial components involved in amylase binding, the alkali extract was subjected to affinity chromatography on amylase-Sepharose. Immunoblotting with a rabbit antiserum against S. gordonii G9B revealed that a 20-kDa streptococcal component was eluted from the amylase-Sepharose with 1% sodium dodecyl sulfate (SDS), 2 M KSCN, or 0.1 M sodium citrate buffer, pH 4.5. Subsequently, the 20-kDa component was prepared from alkali extracts by electroelution from preparative SDS electrophoresis or by gel filtration chromatography. This component was trypsin sensitive, and an antibody raised against it inhibited the binding of I-125-amylase to S. gordonii G9B. Indirect immunofluorescence microscopy and immunogold electron microscopy demonstrated that both bound amylase and the 20-kDa component were localized to the cell division septum on dividing cells or to polar zones on single cells. In addition, exponentially growing bacteria bound more I-125-amylase than stationary-phase cells did. Collectively, these results suggest that a 20-kDa amylase-binding component is present on the surface of the nascent streptococcal cell wall.

引用

页码：4726 / 4733

页数：8

共 47 条

[1] IMMUNOCHEMICAL QUANTITATION OF ALPHA-AMYLASE AND SECRETORY IGA IN PAROTID-SALIVA FROM PEOPLE OF VARIOUS AGES [J].

AGUIRRE, A ;

LEVINE, MJ ;

COHEN, RE ;

TABAK, LA .

ARCHIVES OF ORAL BIOLOGY, 1987, 32 (04) :297-301

[2] CHARACTERIZATION OF INVIVO SALIVARY-DERIVED ENAMEL PELLICLE [J].

ALHASHIMI, I ;

LEVINE, MJ .

ARCHIVES OF ORAL BIOLOGY, 1989, 34 (04) :289-295

[3] USE OF THE PHOTOAFFINITY CROSS-LINKING AGENT N-HYDROXYSUCCINIMIDYL-4-AZIDOSALICYLIC ACID TO CHARACTERIZE SALIVARY-GLYCOPROTEIN BACTERIAL INTERACTIONS [J].

BERGEY, EJ ;

LEVINE, MJ ;

REDDY, MS ;

BRADWAY, SD ;

ALHASHIMI, I .

BIOCHEMICAL JOURNAL, 1986, 234 (01) :43-48

[4]

BIRKHED D, 1978, SCAND J DENT RES, V86, P248

[5]

BURNETTE WN, 1981, ANAL BIOCHEM, V112, P195, DOI 10.1016/0003-2697(81)90281-5

[6]

Carlsson J, 1965, Odontol Revy, V16, P348

[7]

DEMUTH DR, 1990, J BIOL CHEM, V265, P7120

[8] SALIVA-MEDIATED AGGREGATION OF ENTEROCOCCUS-FAECALIS TRANSFORMED WITH A STREPTOCOCCUS-SANGUIS GENE ENCODING THE SSP-5 SURFACE-ANTIGEN [J].

DEMUTH, DR ;

BERTHOLD, P ;

LEBOY, PS ;

GOLUB, EE ;

DAVIS, CA ;

MALAMUD, D .

INFECTION AND IMMUNITY, 1989, 57 (05) :1470-1475

[9] CLONING AND EXPRESSION OF A STREPTOCOCCUS-SANGUIS SURFACE-ANTIGEN THAT INTERACTS WITH A HUMAN SALIVARY AGGLUTININ [J].

DEMUTH, DR ;

DAVIS, CA ;

CORNER, AM ;

LAMONT, RJ ;

LEBOY, PS ;

MALAMUD, D .

INFECTION AND IMMUNITY, 1988, 56 (09) :2484-2490

[10] IMMUNOCHEMICAL STUDY OF HOST PROTEINS IN HUMAN SUPRAGINGIVAL COMPARED WITH DENTURE PLAQUE [J].

DIPAOLA, C ;

HERRERA, MS ;

MANDEL, ID .

ARCHIVES OF ORAL BIOLOGY, 1984, 29 (02) :161-163

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