Complement regulation in the rat glomerulus: Crry and CD59 regulate complement in glomerular mesangial and endothelial cells
RJ Quigg, BP Morgan, VM Holers, S Adler… - Kidney international, 1995 - Elsevier
RJ Quigg, BP Morgan, VM Holers, S Adler, AE Sneed III, CF Lo
Kidney international, 1995•ElsevierComplement regulation in the rat glomerulus: Crry and CD59 regulate complement in
glomerular mesangial and endothelial cells. The complement regulators, decay accelerating
factor, membrane cofactor protein, and CD59 are present in human glomeruli. Crry is the
rodent analogue to the former two proteins. In this study, we examined complement
regulation in cultured rat glomerular endothelial cells (GEnC) and mesangial cells (MES).
Immunoprecipitation of 125 I-labeled membrane proteins and Western blotting studies were …
glomerular mesangial and endothelial cells. The complement regulators, decay accelerating
factor, membrane cofactor protein, and CD59 are present in human glomeruli. Crry is the
rodent analogue to the former two proteins. In this study, we examined complement
regulation in cultured rat glomerular endothelial cells (GEnC) and mesangial cells (MES).
Immunoprecipitation of 125 I-labeled membrane proteins and Western blotting studies were …
Complement regulation in the rat glomerulus: Crry and CD59 regulate complement in glomerular mesangial and endothelial cells. The complement regulators, decay accelerating factor, membrane cofactor protein, and CD59 are present in human glomeruli. Crry is the rodent analogue to the former two proteins. In this study, we examined complement regulation in cultured rat glomerular endothelial cells (GEnC) and mesangial cells (MES). Immunoprecipitation of 125I-labeled membrane proteins and Western blotting studies were performed with anti-Crry and anti-CD59. In both GEnC and MES, Crry was present as 53, 65, and 78 kD proteins. The 20 kD CD59 was apparent in GEnC. CD59 was also present in MES, but in relatively smaller quantities. By Northern analyses, 1.8 kb CD59 mRNA was present in GEnC as well as in RNA from isolated fat glomeruli. mRNA for Crry was present in both GEnC and MES as 2.2 kb species. The functional significance of these proteins was evaluated next. Anti-Thy 1.1 IgG was used to activate the complement classical pathway in MES. To inhibit the function of the complement regulators, anti-CD59 and/or anti-Crry F(ab′)2 antibodies were added with anti-Thy 1.1. Inhibition of Crry function led to enhanced cytotoxicity, while there was no effect when CD59 function was inhibited. The complement alternative pathway was studied by adding complement in Mg-EGTA buffer. Inhibition of Crry led to productive alternative pathway activation, which was accentuated by anti-CD59 when Crry was incompletely inhibited. Alternative pathway regulation was also evaluated in GEnC. Inhibition of CD59 function alone had no effect in GEnC, while inhibition of Crry led to significant cytotoxicity from alternative pathway activation. Under conditions in which Crry was inactive, inhibition of CD59 further enhanced cytotoxicity. Therefore, Crry is present in both GEnC and MES and restricts the complement alternative pathway in both cell types. Crry also regulates the classical pathway in MES. CD59 is present and functionally active in GEnC, while it appears to have a minor role in MES.
Elsevier