GDM seems associated with low l-arginine transport (Figure 4), but higher expression of hCAT-1 in hPMEC, and insulin reverses these effects of the disease selleck chemicals to values in cells from normal pregnancies [65]. Thus, we hypothesize that insulin could be a key factor mediating reversal of the GDM deleterious effect in hPMEC to a phenotype resembling that in cells from normal pregnancies. Adenosine uptake is reduced in hPMEC primary cultures from GDM pregnancies, a phenomenon that has been proposed
as an explanation, at least in part, of the increased vein and whole plasma adenosine concentration detected in this disease [71]. Adenosine uptake in hPMEC is mediated via hENT1 and hENT2 in a similar proportion [30, 71] suggesting that under normal
conditions these two transport mechanisms could share a role in controlling the extracellular levels of adenosine in the human placenta microcirculation. Interestingly, reduced hENT1 and hENT2 expression and activity in hPMEC from GMD pregnancies compared with cells from normal pregnancies is reported [71]. This effect of GDM was most likely due to reduced expression of SLC29A1 and SLC29A2 (for hENT2) in this cell type. Since SLC29A2 promoter transcriptional activity is reduced in hPMEC from GDM pregnancies and the p42/p44mapk/Akt activity Selleck Deforolimus ratio was <1 instead of a predominant mitogenic signaling pathway (i.e., p42/p44mapk/Akt activity ratio >1), a potential metabolic phenotype will predominate in hPMEC from GDM pregnancies [71]. There are no studies addressing the potential modulatory action
of adenosine on the l-arginine/NO pathway in the microcirculation of the human placenta in normal or GDM pregnancies [39, 81]. Preliminary studies suggest that adenosine could acts BCKDHB as modulator of l-arginine transport in hPMEC from normal pregnancies, a phenomenon that seems to require A2AAR and A2BAR activation in this cell type (E Guzmán-Gutiérrez and L Sobrevia, unpublished observations). However, in cells from GDM pregnancies l-arginine transport was lower compared with cells from normal pregnancies, a phenomenon that was further reduced by the use of A2AAR, but not A2BAR antagonists. Thus, GDM is a condition potentially associated with reduced activity of the microvascular endothelial l-arginine/NO pathway due to tonic activation of A2BAR. However, we have recently reported that adenosine also causes vasodilation of human chorionic stem villi vein rings via a mechanism that require endothelium-derived NO [85]. Thus, adenosine is a vasodilator at the microcirculation of the human placenta from normal pregnancies (Figure 5). Since NO synthesis in human fetoplacental endothelium seems to require l-arginine uptake, it is likely that adenosine vasodilation also involved a likely increase in the l-arginine/NO pathway in cells from normal pregnancies.