Phthalates Biomarker Identification and Exposure Estimates in a Population of Pregnant Women

Phthalates are known reproductive and developmental toxicants in experimental animals. However, in humans, there are few data on the exposure of pregnant women that can be used to assess the potential developmental exposure experienced by the fetus. We measured several phthalate metabolites in maternal urine, maternal serum, and cord serum samples collected at the time of delivery from 150 pregnant women from central New Jersey. The urinary concentrations of most metabolites were comparable to or less than among the U.S. general population, except for mono(2-ethylhexyl) phthalate (MEHP), mono(2-ethyl-5-hydroxyhexyl) phthalate (MEHHP), and mono(2-ethyl-5-oxohexyl) phthalate (MEOHP), three metabolites of di(2-ethylhexyl) phthalate (DEHP). The median urinary concentrations of MEHHP (109 μ g/l) and MEOHP (95.1 μ g/l) were more than 5 times their population-based concentrations, whereas the median urinary concentration of MEHP was more than 20 times higher. High concentration of MEHP may indicate a recent exposure to the parent chemical DEHP in the hospital shortly before the collection of the samples. Calculation of daily intakes using the urinary biomarker data reveals that none of the pregnant women tested had integrated exposures to DEHP greater than the Agency for Toxic Substances and Disease Registry's minimal risk levels (MRLs chronic 60, intermediate 100 μ g/kg/day). No abnormal birth outcomes (e.g., birth weight, Apgar Score, and gestational age) were noted in those newborns whose mothers had relatively greater exposure to DEHP during the perinatal period than others in this study. Significantly greater concentrations and detection frequencies in maternal urine than in maternal serum and cord serum suggest that the urinary concentrations of the phthalate metabolites may be more reliable biomarkers of exposure than their concentrations in other biological specimens.     

Bulk Flow Revisited: Transport of a Soluble Protein in the Secretory Pathway

The C-terminal domain, Cp, of the Semliki Forest virus capsid protein, known for its rapid, efficient and chaperone-independent folding, was used to measure bulk fluid flow in the secretory pathway of Chinese hamster ovary cells. Being small, nonglycosylated, soluble and cytoplasmic in origin, Cp was not likely to interact with lectins, cargo receptors and retention factors. Using pulse-chase analysis, we observed that translocation into the endoplasmic reticulum resulted in rapid and efficient folding and transport of the newly synthesized Cp protein to the extracellular medium. The first Cp molecules were secreted 15 min after synthesis, which is the fastest transport of a protein so far recorded in mammalian cells. The rate constant of secretion was 1.2% per min, which amounts to an estimated bulk flow rate of about 155 coat protein II (COPII) vesicles per second. Transport was independent of expression level, and blocked by CI-976, brefeldin A and ATP depletion indicating that it depended on COPII vesicle formation, and followed the classical secretory pathway. In polarized Madin-Darby canine kidney cells, the secretion rate was similar but occurred mainly apically. The results demonstrated that fluid flow in the secretory pathway is fast, and can therefore play a significant role in the secretion of soluble secretory products.     

Secretion of Hedgehog-Related Peptides and WNT During Caenorhabditis elegans Development

There is growing awareness that endocytic trafficking plays a critical role in cell–cell communication during animal development. We are beginning to understand how endocytosis can initiate, modulate or terminate signaling. In contrast, our knowledge of the mechanisms involved in secreting signaling peptides remains more limited, particularly when it comes to secretion at the apical surface in epithelial cells. In this study, we review the mechanisms that control secretion in Caenorhabditis elegans , focusing on the role of Patched family members and the V0 complex of the vacuolar-adenosine triphosphatase (V-ATPase) in secreting Hedgehog-related peptides and of MIG-14/Wls and the retromer complex in secreting EGL-20/WNT.     

Post-Golgi Traffic in Plants

Secretory and endocytic traffic through the post-Golgi endomembrane system regulates the abundance of plasma-membrane proteins such as receptors, transporters and ion channels, modulating the ability of a cell to communicate with its neighbours and to adapt to a changing environment. The major post-Golgi compartments are numerous and appear to be similar to their counterparts in animals. However, endosomes are rather ill defined morphologically but seem to be involved in specific trafficking pathways. Many plasma-membrane proteins cycle constitutively via endosomal compartments. The trans -Golgi network (TGN) appears to be an early endosome where secretory and endocytic traffic meet. Endocytosed proteins that are to be degraded are targeted to the vacuole via the multivesiculate prevacuolar compartment (PVC) whereas cycling proteins pass through recycling endosomes. The trafficking machinery involves the same classes of proteins as in other eukaryotes. However, there are modifications that match the specifics of post-Golgi traffic in plants. Although plants lack epithelia, some plasma-membrane proteins are located on specific faces of the cell which reflects polarized traffic and influences the physiological performance of the tissue. Plants also differentiate highly polarized tip-growing cells in which post-Golgi traffic is adapted to very high rates of targeted exocytosis, endocytosis and recycling.     

Changes in islet plasma membrane calcium-ATPase activity and isoform expression induced by insulin resistance

We studied the effect of insulin resistance (IR) induced by administration of a fructose-rich diet (FRD) to normal Wistar rats for 21 days, upon islet plasma membrane calcium ATPases (PMCAs) and insulin secretion. FRD rats showed significantly higher triglyceride and insulin levels, insulin:glucose ratio and HOMA-IR index than controls. FRD islets released significantly more insulin in response to glucose and showed (a) marked changes in PMCA isoform protein content (decreased PMCA 2 and increased PMCA 3), (b) a decrease in total PMCAs activity, and (c) higher levels of cytosolic calcium [Ca²⁺]_i. The lower PMCAs activity with the resultant increase in [Ca²⁺]_i would favor the compensatory greater release of insulin necessary to cope with the IR state present in FRD rats and to maintain normal glucose homeostasis. Thus, changes in PMCAs activity and isoform expression play a modulatory role upon insulin secretion during long-term adaptation to an increased hormone demand.     

A combination of ultrahigh throughput PathHunter and cytokine secretion assays to identify glucocorticoid receptor agonists

The use of ultrahigh throughput screens (uHTS) is a well-accepted mechanism to identify agonists and antagonists of target receptors. We used the Path Hunter [Path Hunter technology is a registered trademark of DiscoveRx Corporation.] technology from DiscoveRx to screen the entire Merck compound library for glucocorticoid receptor (GR) agonists in a 2.2-μl total reaction volume assayed in a 3456-well plate format. This single addition, homogenous assay which utilizes the principle of enzyme fragment complementation (EFC) to detect nuclear translocation of GR, an initial step of receptor activation, was used to successfully screen a large library of small molecules as indicated by an average signal to background ratio of approximately 4-fold and an average Z-factor value of 0.45. Hits from the HTS campaign were studied in a cytokine secretion assay in primary human monocytes to gain functional information regarding these compounds in a phenotypic and physiologically relevant setting. Our data indicate that using the PathHunter assay, we successfully identified compounds that showed agonism for the GR receptor in primary human monocytes and due to their performance in a physiologically relevant model they likely will have a better chance to evoke clinical efficacy.     

The agglutination protein AggA from Shewanella oneidensis MR-1 is a TolC-like protein and forms active channels in vitro

Type I secretion systems (TISS) are associated with the virulence of Gram-negative bacteria and the secretion of pathogenic molecular determinants. The Shewanella oneidensis MR-1 outer-membrane protein AggA is part of a TISS. Recombinant AggA expressed in Escherichia coli as inclusion bodies can be efficiently refolded in vitro, and can form active channel-tunnels as shown by proteoliposome swelling assays and electrophysiological measurements in lipid bilayers. Structure-based sequence alignments identify AggA as a TolC-like protein, and point to a conserved structural framework among such proteins despite their marginal sequence similarity. Phylogenetic analysis reveals that clustering of TolC-like proteins can be correlated with their involvement in TISS, Resistance/Nodulation/Division (RND) or Major Facilitator Superfamily (MFS) complexes. Taken together, our results establish a first set of structure-function relationships for a bacterial outer-membrane protein likely to be exclusively involved in TISS, and may contribute towards a more accurate classification of Outer-Membrane Factor (OMF) family proteins.     

Diet and reproduction in the Australian butterfly ray Gymnura australis from northern and north‐eastern Australia

The diet of Gymnura australis was dominated by teleosts (99·8% index of relative importance). A wide‐ranging species, females matured at 446 mm disc width (W_D), had a single functional ovary and two functional uteri. Males matured at 377 mm W_D and had a single functional testis.     

Trumpeter Swan Abundance and Growth Rates in Yellowstone National Park

ABSTRACT Decreasing abundance of resident, nonmigratory trumpeter swans (Cygnus buccinator) in Yellowstone National Park (YNP), USA, raised concern that this population, which helped facilitate the restoration of the species across North America, may disappear. We quantified trends in abundance of resident and migratory trumpeter swans in YNP from 1967 to 2007 and investigated the potential mechanisms for declining population trends, including cessation of the supplemental feeding program and relocation programs outside of YNP, density dependence, and annual variations in environmental conditions. Estimated abundance of resident trumpeter swans in YNP ranged from 59 individuals in 1968 to 10 individuals in 2007. Using log-linear modeling, the best approximating model chosen from an a priori set of competing models estimated the annual growth rate (r) of resident swans from 1967 to 2007 was −0.036 (95% CI =−0.042 to −0.030, Akaike wt [w_i] = 0.44). A competing model provided evidence that decreases in abundance became more dramatic after supplemental feeding of grain outside of YNP was terminated in winter 1992–1993 (r̂_1967–1992 = −0.027, 95% CI = −0.039 to −0.015; r̂_1993–2007 = −0.053, 95% CI = −0.029 to −0.080; w_i = 0.42). There was little evidence of density-dependent effects on the resident population growth rates (βYNP_pop = 0.006, 95% CI = −0.017 to 0.007), but rates were lower following severe winters, wetter springs, and warmer summers. Our results indicate that the YNP population of trumpeter swans is decreasing and may act as a sink to surrounding populations. Thus, population levels of YNP trumpeter swans may depend on management outside the Park and we recommend the National Park Service collaborate with surrounding agencies in managing trumpeter swans throughout the Tri-state region where more productive habitats may exist.