Genetic and cellular evidence of vascular inflammation in neurofibromin-deficient mice and humans
Elisabeth A. Lasater, Fang Li, Waylan K. Bessler, Myka L. Estes, Sasidhar Vemula, Cynthia M. Hingtgen, Mary C. Dinauer, Reuben Kapur, Simon J. Conway, David A. Ingram Jr.
Elisabeth A. Lasater, Fang Li, Waylan K. Bessler, Myka L. Estes, Sasidhar Vemula, Cynthia M. Hingtgen, Mary C. Dinauer, Reuben Kapur, Simon J. Conway, David A. Ingram Jr.
View: Text | PDF
Research Article Vascular biology

Genetic and cellular evidence of vascular inflammation in neurofibromin-deficient mice and humans

Abstract

Neurofibromatosis type 1 (NF1) results from mutations in the NF1 tumor suppressor gene, which encodes the protein neurofibromin. NF1 patients display diverse clinical manifestations, including vascular disease, which results from neointima formation and vessel occlusion. However, the pathogenesis of NF1 vascular disease remains unclear. Vessel wall homeostasis is maintained by complex interactions between vascular and bone marrow–derived cells (BMDCs), and neurofibromin regulates the function of each cell type. Therefore, utilizing cre/lox techniques and hematopoietic stem cell transplantation to delete 1 allele of Nf1 in endothelial cells, vascular smooth muscle cells, and BMDCs alone, we determined which cell lineage is critical for neointima formation in vivo in mice. Here we demonstrate that heterozygous inactivation of Nf1 in BMDCs alone was necessary and sufficient for neointima formation after vascular injury and provide evidence of vascular inflammation in Nf1+/– mice. Further, analysis of peripheral blood from NF1 patients without overt vascular disease revealed increased concentrations of inflammatory cells and cytokines previously linked to vascular inflammation and vasoocclusive disease. These data provide genetic and cellular evidence of vascular inflammation in NF1 patients and Nf1+/– mice and provide a framework for understanding the pathogenesis of NF1 vasculopathy and potential therapeutic and diagnostic interventions.

Authors

Elisabeth A. Lasater, Fang Li, Waylan K. Bessler, Myka L. Estes, Sasidhar Vemula, Cynthia M. Hingtgen, Mary C. Dinauer, Reuben Kapur, Simon J. Conway, David A. Ingram Jr.

×

Figure 1

Histological and morphometric analysis of WT, Nf1+/–, Nf1fl/+;Tie2cre, and Nf1fl/+;SM22cre mice.

Options: View larger image (or click on image) Download as PowerPoint
Histological and morphometric analysis of WT, Nf1+/–, Nf1fl/+;Tie2cre, a...
(A) Representative H&E-stained cross sections of uninjured and injured carotid arteries from WT, Nf1+/–, Nf1fl/+;Tie2cre, and Nf1fl/+;SM22cre mice. Red arrows indicate neointima boundaries. Scale bars: 50 μm. (B and C) Quantification of neointima area (B) and I/M ratio (C) of uninjured (white bars) and injured (black bars) carotid arteries from WT, Nf1+/–, Nf1fl/+;Tie2cre, and Nf1fl/+;SM22cre mice. Data represent the mean of 3 arterial cross sections (400, 800, and 1,200 μm proximal to the ligation) ± SEM, n = 4–7. *P < 0.001 for Nf1+/– uninjured versus Nf1+/– injured and for Nf1+/– injured versus WT injured, Nf1fl/+;Tie2cre injured, and Nf1fl/+;SM22cre injured, by 1-way ANOVA with Tukey’s post-hoc test.