Figure 4.
Figure 4. Parasympathetic deficiency increases nocturnal HSPC BM adhesion and homing through β2 -adrenergic signaling in the microenvironment. Vcam1 (A), Sele (B), and Selp (C) mRNA expression at ZT13 in the unfractionated BM of control Gfra2+/− mice, Gfra2−/− mice, single β2-AR (Adrb2)-deficient or β3-AR (Adrb3)-deficient mice, or compound Gfra2−/−Adrb2−/− and Gfra2−/−Adrb3−/− mice. Vcam1 (D), Sele (E), and Selp (F) mRNA expression at ZT13 in CD45−Ter119− endothelial (CD31+) or nonendothelial (CD31−) cells from Gfra2−/− and control Gfra2+/− mice. (G) Scheme showing the protocol used for blockade of in vivo HSPC adhesion to blood vessels using antibodies against α4-integrin, P-selectin, and E-selectin (IV injection at ZT11 and analysis at ZT13). (H) HSPCs circulating at ZT13, 2 hours after injection of blocking antibodies (Abs) or control IgG. Please note that CFU-C fold change goes from a 3.2-fold increase in control immunoglobulin G–treated mice to a 1.3-fold increase in blocking antibody–treated mice. (I) Frequencies of donor-derived WT CD45.1+ lin−sca1+ckit+ HSPCs at ZT2 that homed during the night to the BM after IV transplantation (at ZT10) into nonirradiated Gfra2−/− mice or control Gfra2+/− mice preconditioned with saline or β2 adrenergic antagonist (ICI118,551) 4 hours before transplantation. (A-F,H-I) Data are mean ± standard error of the mean; n (inside bars) and P values (multivariate analysis for >2 groups) are indicated. *P < .05, **P < .01, ***P < .001, 1-way analysis of variance with Bonferroni comparisons. ns, not significant.

Parasympathetic deficiency increases nocturnal HSPC BM adhesion and homing through β2-adrenergic signaling in the microenvironment.Vcam1 (A), Sele (B), and Selp (C) mRNA expression at ZT13 in the unfractionated BM of control Gfra2+/− mice, Gfra2−/− mice, single β2-AR (Adrb2)-deficient or β3-AR (Adrb3)-deficient mice, or compound Gfra2−/−Adrb2−/− and Gfra2−/−Adrb3−/− mice. Vcam1 (D), Sele (E), and Selp (F) mRNA expression at ZT13 in CD45Ter119 endothelial (CD31+) or nonendothelial (CD31) cells from Gfra2−/− and control Gfra2+/− mice. (G) Scheme showing the protocol used for blockade of in vivo HSPC adhesion to blood vessels using antibodies against α4-integrin, P-selectin, and E-selectin (IV injection at ZT11 and analysis at ZT13). (H) HSPCs circulating at ZT13, 2 hours after injection of blocking antibodies (Abs) or control IgG. Please note that CFU-C fold change goes from a 3.2-fold increase in control immunoglobulin G–treated mice to a 1.3-fold increase in blocking antibody–treated mice. (I) Frequencies of donor-derived WT CD45.1+ linsca1+ckit+ HSPCs at ZT2 that homed during the night to the BM after IV transplantation (at ZT10) into nonirradiated Gfra2−/− mice or control Gfra2+/− mice preconditioned with saline or β2 adrenergic antagonist (ICI118,551) 4 hours before transplantation. (A-F,H-I) Data are mean ± standard error of the mean; n (inside bars) and P values (multivariate analysis for >2 groups) are indicated. *P < .05, **P < .01, ***P < .001, 1-way analysis of variance with Bonferroni comparisons. ns, not significant.

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