Barbara E. Dreyer
Yale University
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Publication
Featured researches published by Barbara E. Dreyer.
Journal of Bone and Mineral Research | 2005
Xuesong Chen; Carolyn M. Macica; Barbara E. Dreyer; Vicki E. Hammond; Julie R Hens; William M. Philbrick; Arthur E. Broadus
The PTHrP gene generates low‐abundance mRNA and protein products that are not easily localized by in situ hybridization histochemistry or immunohistochemistry. We report here a PTHrP‐lacZ knockin mouse in which β‐gal activity seems to provide a simple and sensitive read‐out of PTHrP gene expression.
Biochemical and Biophysical Research Communications | 1989
Kyoji Ikeda; Eleanor C. Weir; Kazushige Sakaguchi; William J. Burtis; Mark B. Zimering; Marguerite Mangin; Barbara E. Dreyer; Maria Luisa Brandi; G. D. Aurbach; Arthur E. Broadus
A novel parathyroid hormone-related peptide has been identified in tumors associated with the syndrome of humoral hypercalcemia of malignancy. Subsequently, mRNAs encoding this peptide have been found to be expressed in a number of normal tissues, including the parathyroids. Using Northern blotting, RNase protection, and immunochemical techniques, we examined a clonal rat parathyroid cell line originally developed as a model system for studying parathyroid cell physiology. We found that this line expresses the parathyroid hormone-related peptide but not parathyroid hormone itself. Secretion of the parathyroid hormone-related peptide varied inversely with extracellular calcium concentration, but neither calcium nor 1,25-dihydroxyvitamin D3 appeared to influence steady-state parathyroid hormone-related peptide mRNA levels. This clonal line may prove to be an interesting system for studying the factors responsible for tissue-specific parathyroid hormone and parathyroid hormone-related peptide gene expression.
Journal of Neurochemistry | 2008
Elizabeth H. Holt; Charles Lu; Barbara E. Dreyer; Priscilla S. Dannies; Arthur E. Broadus
The parathyroid hormone‐related peptide (PTHrP) gene has been reported to be subject to a wide variety of physiological and pharmacological controls. Two distinct patterns of PTHrP mRNA response have been recognized, one characterized by a prolonged or plateau response lasting many hours to days and the second characterized by rapid induction‐deinduction kinetics and lasting 1 to several hours. The kinetics of the second pattern are similar to those displayed by primary response genes like nuclear protooncogenes, cytokines, and growth factors. In GH4C1, rat pituitary cells, 17β‐estradiol induced a rapid and transient increase in PTHrP mRNA expression, with a peak response at 1–2 h. This response appeared to be due to a rapid and transient burst in gene transcription, which by runoff analysis was maximal at 20–40 min and declined thereafter. PTHrP mRNA half‐life was 30 min in these cells and was unaltered by estradiol. Cy‐cloheximide did not block the 17β‐estradiol‐induced response but rather prolonged it, and runoff analysis revealed that this effect was due to a prolongation or persistence of PTHrP gene transcription. These findings suggest that the transient nature of the native response reflects the effects of an estrogen‐inducible represser. All of these features are characteristic of a prototypical primary response gene.
Brain Research | 2002
Oindrila Chatterjee; Inaam A. Nakchbandi; William M. Philbrick; Barbara E. Dreyer; Jian-Ping Zhang; Leonard K. Kaczmarek; Michael Brines; Arthur E. Broadus
Parathyroid hormone-related protein (PTHrP) was discovered a dozen years ago as a product of malignant tumors. It is now known that PTHrP is a paracrine factor with multiple biological functions. One such function is to relax smooth muscle by inhibiting calcium influx into the cell. In the central nervous system, PTHrP and its receptor are widely expressed in neurons in the cerebral cortex, hippocampus and cerebellum. The function of PTHrP in the CNS is not known. Previous work has shown that expression of the PTHrP gene is depolarization-dependent in cultured cerebellar granule cells and depends specifically on L-type voltage sensitive calcium channel (L-VSCC) Ca(2+) influx. PTHrP has also been found to be capable of protecting these cells against kainic acid-induced excitotoxicity. Here, we tested the idea that mice with a PTHrP-null CNS might display hypersensitivity to kainic acid excitotoxicity. We found that these mice were six-fold more sensitive than control littermate mice to kainic-acid-induced seizures as well as hippocampal c-Fos expression. PTHrP-null embryonic mixed cerebral cortical cultures were more sensitive to kainic acid than control cultures, and PTHrP addition was found to be protective against kainate toxicity in both PTHrP-null and control cultures. By whole-cell techniques, PTHrP was found to reduce L-VSCC Ca(2+) influx in cultured mouse neuroblastoma cells. We conclude that PTHrP functions as a component of a neuroprotective feedback loop that is structured around the L-type calcium channel. This loop appears to be operative in vivo as well as in vitro.
Proceedings of the National Academy of Sciences of the United States of America | 1998
William M. Philbrick; Barbara E. Dreyer; Inaam A. Nakchbandi; Andrew C. Karaplis
Development | 2001
John Foley; Pamela Dann; James Hong; Jason Cosgrove; Barbara E. Dreyer; David L. Rimm; Maureen E. Dunbar; William M. Philbrick; John J. Wysolmerski
The New England Journal of Medicine | 1984
Arthur E. Broadus; Karl L. Insogna; Robert Lang; Alice F. Ellison; Barbara E. Dreyer
Proceedings of the National Academy of Sciences of the United States of America | 1989
Marguerite Mangin; Kyoji Ikeda; Barbara E. Dreyer; Arthur E. Broadus
The Journal of Clinical Endocrinology and Metabolism | 1985
Karl L. Insogna; Arthur E. Broadus; Barbara E. Dreyer; Alice F. Ellison; Joseph M. Gertner
Journal of Investigative Dermatology | 1998
John Foley; John J. Wysolmerski; Barbara E. Dreyer; Arthur E. Broadus; William M. Philbrick; B. Jack Longely
