Search Results

You are looking at 1 - 3 of 3 items for

  • Author: T Rice x
  • Refine by access: All content x
Clear All Modify Search
W Farrugia
Search for other papers by W Farrugia in
Google Scholar
PubMed
Close
,
T de Gooyer
Search for other papers by T de Gooyer in
Google Scholar
PubMed
Close
,
GE Rice
Search for other papers by GE Rice in
Google Scholar
PubMed
Close
,
JM Moseley
Search for other papers by JM Moseley in
Google Scholar
PubMed
Close
, and
ME Wlodek
Search for other papers by ME Wlodek in
Google Scholar
PubMed
Close

The placental syncytiotrophoblast is the site for mineral and nutrient exchange across the maternal-fetal interface. It has been proposed that parathyroid hormone-related protein (PTHrP) is a key factor in the maintenance of a maternal-fetal calcium gradient. Using simultaneously prepared microvillous (maternal facing) and basal (fetal facing) syncytiotrophoblast membranes from term human placentae (n=8), we determined the relative contribution of PTH(1-34), PTHrP(1-34) and PTHrP(67-94) to the regulation of syncytiotrophoblast calcium efflux. The vesicles had correct right-side-out membrane orientation and specific markers validated the fractionation of microvillous and basal membrane vesicles. Calcium efflux was studied by preloading vesicles with calcium-45 in the presence of calcium and magnesium and then incubating the vesicles at 37 degrees C for 15 min with the peptides. In basal membranes, PTHrP(1-! 34) significantly stimulated calcium efflux at a dose of 12.5 nmol/l, whereas PTH(1-34)-stimulated efflux was significant at 50 nmol/l (P<0.05, ANOVA). This efflux was significantly reduced in the presence of the PTH/PTHrP receptor antagonist (PTHrP(7-34)). Midmolecule PTHrP(67-94) had no significant effect on basal membrane calcium efflux. PTH(1-34), PTHrP(1-34) or PTHrP(67-94) had no significant effects on MVM calcium efflux. This study, using the human syncytiotrophoblast in vitro membrane system, demonstrated that PTHrP(1-34) and PTH(1-34) stimulate calcium transport across the basal, but not microvillous, syncytiotrophoblast membrane vesicles, mediated via the PTH/PTHrP receptor.

Free access
Y Hong
Search for other papers by Y Hong in
Google Scholar
PubMed
Close
,
J Gagnon
Search for other papers by J Gagnon in
Google Scholar
PubMed
Close
,
T Rice
Search for other papers by T Rice in
Google Scholar
PubMed
Close
,
L Perusse
Search for other papers by L Perusse in
Google Scholar
PubMed
Close
,
AS Leon
Search for other papers by AS Leon in
Google Scholar
PubMed
Close
,
JS Skinner
Search for other papers by JS Skinner in
Google Scholar
PubMed
Close
,
JH Wilmore
Search for other papers by JH Wilmore in
Google Scholar
PubMed
Close
,
C Bouchard
Search for other papers by C Bouchard in
Google Scholar
PubMed
Close
, and
DC Rao
Search for other papers by DC Rao in
Google Scholar
PubMed
Close

Familial correlation analyses were used to evaluate the familial aggregation of plasma androgens and androgen glucuronides (testosterone (TESTO), dihydrotestosterone (DHT), androstane-3 alpha,17 beta-diol glucuronide (3 alpha-DIOL-G), and androsterone glucuronide (ADT-G)) in 505 members of 99 white families and 296 members of 111 black families participating in the Health, Risk Factors, Exercise Training and Genetics (HERITAGE) Family Study. Each of these four measures was determined by RIA after separation of conjugated and unconjugated steroid using C18 column chromatography. All participants were sedentary prior to being including in this study. Significant spouse correlations, as well as parent-offspring and sibling correlations, were found for TESTO, DHT, 3 alpha-DIOL-G, and ADT-G in the white sample, suggesting that common familial environments and genes contribute to the familial resemblance. In the black sample, significant sibling and parent-offspring correlations were found for all four phenotypes, while the spouse correlation was marginally significant for 3 alpha-DIOL-G and not significant for TESTO, DHT, and ADT-G. The non-significance of spouse correlations in the black individuals may be due to the small number of spouse pairs. The maximal heritability estimates of TESTO, DHT, 3 alpha-DIOL-G, and ADT-G were 69%, 87%, 74%, and 56% for white individuals and 70%, 73%, 62%, and 48% for black individuals respectively. Sex differences in heritability estimates were found in the white individuals, but they were less dramatic in the black individuals. In conclusion, plasma levels of androgens and androgen glucuronides are highly heritable in both white individuals and black individuals. There are notable sex differences in the white individuals.

Free access
N E Curtis
Search for other papers by N E Curtis in
Google Scholar
PubMed
Close
,
P W M Ho
Search for other papers by P W M Ho in
Google Scholar
PubMed
Close
,
R G King
Search for other papers by R G King in
Google Scholar
PubMed
Close
,
W Farrugia
Search for other papers by W Farrugia in
Google Scholar
PubMed
Close
,
E K Moses
Search for other papers by E K Moses in
Google Scholar
PubMed
Close
,
M T Gillespie
Search for other papers by M T Gillespie in
Google Scholar
PubMed
Close
,
J M Moseley
Search for other papers by J M Moseley in
Google Scholar
PubMed
Close
,
G E Rice
Search for other papers by G E Rice in
Google Scholar
PubMed
Close
, and
M E Wlodek
Search for other papers by M E Wlodek in
Google Scholar
PubMed
Close

Abstract

Parathyroid hormone-related protein (PTHrP) gene expression and/or immunoreactive protein have previously been identified in the uterus and intrauterine gestational tissues. The putative roles of PTHrP during pregnancy include vasodilatation, regulation of placental calcium transfer, uterine smooth muscle relaxation and normal fetal development. The aims of this study were 1) to determine the tissue-specific and temporal expression of PTHrP mRNA and immunoreactive protein in human gestational tissues collected at preterm and term; and 2) to determine the effect of labour on PTHrP expression by collecting these tissues from women undergoing elective caesarean section (before labour), intra-partum caesarean section during spontaneous-onset labour (during labour), and women with spontaneous labour and normal vaginal delivery (after labour). Total RNA and protein were extracted from placenta, amnion (over placenta and reflected) and choriodecidua for analysis by Northern blot (using a specific human PTHrP cDNA probe), and by N-terminal PTHrP RIA respectively. In amnion over placenta, reflected amnion and choriodecidua both PTHrP mRNA relative abundance and immunoreactive protein were significantly elevated at term compared with preterm (P<0·01). At term, both PTHrP and its mRNA were significantly greater in amnion than in placenta and choriodecidua (P<0·05). Also, both PTHrP and its mRNA were significantly elevated in amnion over placenta compared with reflected amnion (P<0·05). The expression of PTHrP and its mRNA did not change in association with term labour or rupture of the fetal membranes, therefore this study provides no evidence for a specific PTHrP role in the onset and/or maintenance of term labour. However, the significant up-regulation of PTHrP mRNA and protein in the fetal membranes at term compared with preterm suggests an important role in late human pregnancy.

Journal of Endocrinology (1997) 154, 103–112

Restricted access