In this study, we did not www.selleckchem.com/products/AC-220.html explore the relationship between these mechanisms and estrogens; however they must be taken into account in the overall scenario, as also shown by the more severe phenotype of female mice. A number of clinical observations35 indicate that estrogens play a role in polycystic liver diseases. Estrogen receptor-β is up-regulated in liver cysts of ADPKD patients, and 17-β-estradiol stimulates the proliferation of cystic cholangiocytes obtained from patients with ADPKD; this has also shown that ADPKD epithelium is sensitive to the proliferative effects of estrogens and IGF1.5 Estrogens
also promote the synthesis and release of growth factors, including IGF1, from the cyst epithelium.5 In conclusion, our study demonstrates that mTOR plays a central role in liver cyst growth in mice with defective PC2 (Fig. 8). The mTOR pathway regulates HIF1α-dependent VEGF secretion and appears central to the proliferative, antiapoptotic, and pro-angiogenic effects of IGF1, one of the major factors generated by the cystic epithelium.
The mTOR inhibitor rapamycin inhibits VEGF secretion and signaling and significantly reduces liver cyst growth by reducing proliferation and increasing apoptosis of the cystic Smad inhibitor epithelium. This study also reveals a mechanistic link between mTOR and ERK and HIF1α-mediated VEGF secretion and provides a proof of concept for the potential use of mTOR inhibitors in polycystic liver disease and in conditions with aberrant cholangiocyte proliferation. Additional Supporting Information may be found in the online version of this article. “
“Cytomegalovirus is a common viral pathogen that influences the outcome of organ transplantation. To date, there is no established method to evaluate the effects of human see more CMV (HCMV) treatments in vivo except for human clinical trials. In the current study, we describe the development of a mouse model that supports the in vivo propagation of HCMV. One million viable human hepatocytes, purified from human livers, were
injected into the spleens of severe combined immunodeficient/albumin linked-urokinase type plasminogen activator transgenic mice. A clinical strain of HCMV was inoculated in mice with confirmed human hepatocyte engraftment or in non-chimeric controls. Infection was monitored through HCMV titers in the plasma. Mice were administrated ganciclovir (50 mg/kg per day, i.p.) beginning at 2 days post-HCMV inoculation, or human liver natural killer (NK) cells (20 × 106 cells/mouse, i.v.) 1 day prior to HCMV inoculation. Chimeric mice that received HCMV showed high plasma titers of HCMV DNA on days 1 and 6 that became undetectable by day 11 post-inoculation. In contrast, non-transplanted mice had only residual plasma inoculum detection at day 1 and no detectable viremia thereafter.