A major role for VCAM-1, but not ICAM-1, in early atherosclerosis
Myron I. Cybulsky, … , Philip W. Connelly, David S. Milstone
Myron I. Cybulsky, … , Philip W. Connelly, David S. Milstone
Published May 15, 2001
Citation Information: J Clin Invest. 2001;107(10):1255-1262. https://doi.org/10.1172/JCI11871.
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Article

A major role for VCAM-1, but not ICAM-1, in early atherosclerosis

Abstract

VCAM-1 and ICAM-1 are endothelial adhesion molecules of the Ig gene superfamily that may participate in atherogenesis by promoting monocyte accumulation in the arterial intima. Both are expressed in regions predisposed to atherosclerosis and at the periphery of established lesions, while ICAM-1 is also expressed more broadly. To evaluate functions of VCAM-1 in chronic disease, we disrupted its fourth Ig domain, producing the murine Vcam1D4D allele. VCAM-1D4D mRNA and protein were reduced to 2–8% of wild-type allele (Vcam1+) levels but were sufficient to partially rescue the lethal phenotype of VCAM-1–null embryos. After crossing into the LDL receptor–null background, Vcam1+/+ and Vcam1D4D/D4D paired littermates were generated from heterozygous intercrosses and fed a cholesterol-enriched diet for 8 weeks. The area of early atherosclerotic lesions in the aorta, quantified by en face oil red O staining, was reduced significantly in Vcam1D4D/D4D mice, although cholesterol levels, lipoprotein profiles, and numbers of circulating leukocytes were comparable to wild-type. In contrast, deficiency of ICAM-1 either alone or in combination with VCAM-1 deficiency did not alter nascent lesion formation. Therefore, although expression of both VCAM-1 and ICAM-1 is upregulated in atherosclerotic lesions, our data indicate that VCAM-1 plays a dominant role in the initiation of atherosclerosis.

Authors

Myron I. Cybulsky, Kaeko Iiyama, Hongmei Li, Suning Zhu, Mian Chen, Motoi Iiyama, Vannessa Davis, Jose-Carlos Gutierrez-Ramos, Philip W. Connelly, David S. Milstone

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Figure 2

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VCAM-1 expression in Vcam1D4D/D4D mice. (a) Northern blot analysis of VC...
VCAM-1 expression in Vcam1D4D/D4D mice. (a) Northern blot analysis of VCAM-1, ICAM-1, and β-actin expression using total or oligo dT–enriched RNA (mRNA) from hearts or lungs of control (C) or LPS-treated Vcam1+/+ (+/+), Vcam1+/D4D (+/D4D), and Vcam1D4D/D4D (D4D/D4D) mice. Bars on the right indicate 18S ribosomal RNA migration. Transcripts corresponding to the 7 (asterisks) and 3 (filled diamonds) Ig VCAM-1 were found in Vcam1+/+ and Vcam1+/D4D mice, whereas expression of 6 (arrowheads) and possibly 4 (open circle) Ig domain forms was found in VCAM-1D4D/D4D mice. (b) RT-PCR analysis of 7, 6, and 3 Ig VCAM-1 (7D, 6D, 3D) mRNA in lungs of LPS-treated mice. In Vcam1D4D/D4D mice, domain-specific primers did not detect D4 found in 7 Ig VCAM-1. (c) Immunoprecipitation of cell surface VCAM-1 and ICAM-1 from Vcam1+/+ and Vcam1D4D/D4D biotin-labeled cultured lung endothelial cells. TNF induced expression of 90- to 95-kDa (asterisk) and 36- to 40-kDa (filled diamond) proteins, corresponding to 7 and 3 Ig VCAM-1, in Vcam1+/+ cells, and 80- to 85-kDa (arrowhead) and possibly 50- to 60-kDa (open circle) proteins, corresponding to 6 and 4 Ig VCAM-1 in VCAM-1D4D/D4D cells. No 7 Ig VCAM-1 was detected in VCAM-1D4D/D4D cells. TNF-induced ICAM-1 expression was comparable.