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      Bone Mineral Density Increases in Trans Persons After 1 Year of Hormonal Treatment: A Multicenter Prospective Observational Study : INCREASE OF BMD IN TRANS PERSONS AFTER 1-YEAR CHT

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          Estrogen prevents bone loss via estrogen receptor alpha and induction of Fas ligand in osteoclasts.

          Estrogen prevents osteoporotic bone loss by attenuating bone resorption; however, the molecular basis for this is unknown. Here, we report a critical role for the osteoclastic estrogen receptor alpha (ERalpha) in mediating estrogen-dependent bone maintenance in female mice. We selectively ablated ERalpha in differentiated osteoclasts (ERalpha(DeltaOc/DeltaOc)) and found that ERalpha(DeltaOc/DeltaOc) females, but not males, exhibited trabecular bone loss, similar to the osteoporotic bone phenotype in postmenopausal women. Further, we show that estrogen induced apoptosis and upregulation of Fas ligand (FasL) expression in osteoclasts of the trabecular bones of WT but not ERalpha(DeltaOc/DeltaOc) mice. The expression of ERalpha was also required for the induction of apoptosis by tamoxifen and estrogen in cultured osteoclasts. Our results support a model in which estrogen regulates the life span of mature osteoclasts via the induction of the Fas/FasL system, thereby providing an explanation for the osteoprotective function of estrogen as well as SERMs.
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            Effect of testosterone and estradiol in a man with aromatase deficiency.

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              Accuracy of 6 routine 25-hydroxyvitamin D assays: influence of vitamin D binding protein concentration.

              Recent recognition of its broad pathophysiological importance has triggered an increased interest in 25-hydroxyvitamin D [25(OH)D]. By consequence, throughput in 25(OH)D testing has become an issue for clinical laboratories, and several automated assays for measurement of 25(OH)D are now available. The aim of this study was to test the accuracy and robustness of these assays by comparing their results to those of an isotope dilution/online solid-phase extraction liquid chromatography/tandem mass spectrometry (ID-XLC-MS/MS) method. We put specific focus on the influence of vitamin D-binding protein (DBP) by using samples with various concentrations of DBP. We used 5 automated assays (Architect, Centaur, iSYS, Liaison, and Elecsys), 1 RIA (Diasorin) preceded by extraction, and an ID-XLC-MS/MS method to measure 25(OH)D concentrations in plasma samples of 51 healthy individuals, 52 pregnant women, 50 hemodialysis patients, and 50 intensive care patients. Using ELISA, we also measured DBP concentrations in these samples. Most of the examined 25(OH)D assays showed significant deviations in 25(OH)D concentrations from those of the ID-XLC-MS/MS method. As expected, DBP concentrations were higher in samples of pregnant women and lower in samples of IC patients compared to healthy controls. In 4 of the 5 fully automated 25(OH)D assays, we observed an inverse relationship between DBP concentrations and deviations from the ID-XLC-MS/MS results. 25(OH)D measurements performed with most immunoassays suffer from inaccuracies that are DBP concentration dependent. Therefore, when interpreting results of 25(OH)D measurements, careful consideration of the measurement method is necessary.
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                Author and article information

                Journal
                Journal of Bone and Mineral Research
                J Bone Miner Res
                Wiley
                08840431
                June 2017
                June 2017
                May 02 2017
                : 32
                : 6
                : 1252-1260
                Affiliations
                [1 ]Department of Internal Medicine and Center of Expertise on Gender Dysphoria; VU University Medical Center; Amsterdam the Netherlands
                [2 ]Department of Clinical Chemistry; VU University Medical Center; Amsterdam the Netherlands
                [3 ]Sexual Medicine and Andrology Unit, Department of Experimental, Clinical, and Biomedical Sciences; University of Florence; Florence Italy
                [4 ]Department of Endocrinology; Oslo University Hospital; Oslo Norway
                [5 ]Department of Endocrinology; Center for Sexology and Gender; Ghent University Hospital; Ghent Belgium
                Article
                10.1002/jbmr.3102
                28370342
                8deede27-a4bb-4e2d-8dd7-d2d239d14e7f
                © 2017

                http://doi.wiley.com/10.1002/tdm_license_1.1

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