Your search keyword '"Adams LD"' showing total 92 results

51. RGS5, RGS4, and RGS2 expression and aortic contractibility are dynamically co-regulated during aortic banding-induced hypertrophy.

Author

Wang X, Adams LD, Pabón LM, Mahoney WM Jr, Beaudry D, Gunaje J, Geary RL, Deblois D, and Schwartz SM

Subjects

Animals, Aorta pathology, Blotting, Western, Cells, Cultured, Hypertension metabolism, Hypertension pathology, Hypertension physiopathology, Hypertrophy, In Vitro Techniques, Male, Muscle, Smooth, Vascular metabolism, Muscle, Smooth, Vascular physiopathology, Phenylephrine pharmacology, RGS Proteins genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Rats, Reverse Transcriptase Polymerase Chain Reaction, Serotonin pharmacology, Signal Transduction drug effects, Signal Transduction physiology, Vasoconstriction drug effects, Aorta metabolism, Aorta physiopathology, RGS Proteins metabolism, Vasoconstriction physiology

Abstract

Overexpression of regulator of G protein signaling 5 (RGS5) in arteries over veins is the most striking difference observed using microarray analysis. The obvious question is what arterial function might require RGS5. Based on functions of homologous proteins in regulating cardiac mass and G-protein-coupled receptor (GPCR) signaling, we proposed that RGS5 and vascular expressed RGS2 and RGS4 could participate in regulating arterial hypertrophy. We used the suprarenal abdominal aorta banding model to induce hypertension and hypertrophy. All 3 RGS messages were expressed in unmanipulated aorta with RGS5 predominating. After 2 days, thoracic aorta lost expression of RGS5, 4, and 2. At 1 week, all three returned to normal, and at 28 days, they increased many fold above normal. Valsartan blockade of angiotensin II (angII)/angII type 1 receptor signaling prevented upregulation of RGS messages but only delayed mass increases, implying wall mass regulation involves both angII-dependent and angII-independent pathways. The abdominal aorta showed less dramatic expression changes in RGS5 and 4, but not 2. Again, those changes were delayed by valsartan treatment with no mass changes. Thoracic aorta contraction to GPCR agonists was examined in aortic explant rings to identify vessel wall physiological changes. In 2-day aorta, the response to Galphaq/i agonists increased above normal, while 28-day aorta had attenuated induced contraction via Galphaq/i agonist, implicating a connection between RGS message levels and changes in GPCR-induced contraction. In vitro overexpression studies showed RGS5 inhibits angII-induced signaling in smooth muscle cells. This study is the first experimental evidence that changes in RGS expression and function correlate with vascular remodeling.

Published

2008

52. Capillary regeneration in scleroderma: stem cell therapy reverses phenotype?

Author

Fleming JN, Nash RA, McLeod DO, Fiorentino DF, Shulman HM, Connolly MK, Molitor JA, Henstorf G, Lafyatis R, Pritchard DK, Adams LD, Furst DE, and Schwartz SM

Subjects

Humans, Phenotype, Regeneration, Capillaries physiology, Scleroderma, Diffuse surgery, Stem Cell Transplantation

Abstract

Background: Scleroderma is an autoimmune disease with a characteristic vascular pathology. The vasculopathy associated with scleroderma is one of the major contributors to the clinical manifestations of the disease., Methodology/principal Findings: We used immunohistochemical and mRNA in situ hybridization techniques to characterize this vasculopathy and showed with morphometry that scleroderma has true capillary rarefaction. We compared skin biopsies from 23 scleroderma patients and 24 normal controls and 7 scleroderma patients who had undergone high dose immunosuppressive therapy followed by autologous hematopoietic cell transplant. Along with the loss of capillaries there was a dramatic change in endothelial phenotype in the residual vessels. The molecules defining this phenotype are: vascular endothelial cadherin, a supposedly universal endothelial marker required for tube formation (lost in the scleroderma tissue), antiangiogenic interferon alpha (overexpressed in the scleroderma dermis) and RGS5, a signaling molecule whose expression coincides with the end of branching morphogenesis during development and tumor angiogenesis (also overexpressed in scleroderma skin. Following high dose immunosuppressive therapy, patients experienced clinical improvement and 5 of the 7 patients with scleroderma had increased capillary counts. It was also observed in the same 5 patients, that the interferon alpha and vascular endothelial cadherin had returned to normal as other clinical signs in the skin regressed, and in all 7 patients, RGS5 had returned to normal., Conclusion/significance: These data provide the first objective evidence for loss of vessels in scleroderma and show that this phenomenon is reversible. Coordinate changes in expression of three molecules already implicated in angiogenesis or anti-angiogenesis suggest that control of expression of these three molecules may be the underlying mechanism for at least the vascular component of this disease. Since rarefaction has been little studied, these data may have implications for other diseases characterized by loss of capillaries including hypertension, congestive heart failure and scar formation.

Published

2008

53. CD34 expression by hair follicle stem cells is required for skin tumor development in mice.

Author

Trempus CS, Morris RJ, Ehinger M, Elmore A, Bortner CD, Ito M, Cotsarelis G, Nijhof JG, Peckham J, Flagler N, Kissling G, Humble MM, King LC, Adams LD, Desai D, Amin S, and Tennant RW

Subjects

9,10-Dimethyl-1,2-benzanthracene, Animals, Antigens, CD34 genetics, Cell Cycle physiology, Cell Movement physiology, Female, Hair Follicle pathology, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, Skin Neoplasms chemically induced, Skin Neoplasms pathology, Stem Cells pathology, Tetradecanoylphorbol Acetate, Antigens, CD34 biosynthesis, Hair Follicle metabolism, Skin Neoplasms metabolism, Stem Cells metabolism

Abstract

The cell surface marker CD34 marks mouse hair follicle bulge cells, which have attributes of stem cells, including quiescence and multipotency. Using a CD34 knockout (KO) mouse, we tested the hypothesis that CD34 may participate in tumor development in mice because hair follicle stem cells are thought to be a major target of carcinogens in the two-stage model of mouse skin carcinogenesis. Following initiation with 200 nmol 7,12-dimethylbenz(a)anthracene (DMBA), mice were promoted with 12-O-tetradecanoylphorbol-13-acetate (TPA) for 20 weeks. Under these conditions, CD34KO mice failed to develop papillomas. Increasing the initiating dose of DMBA to 400 nmol resulted in tumor development in the CD34KO mice, albeit with an increased latency and lower tumor yield compared with the wild-type (WT) strain. DNA adduct analysis of keratinocytes from DMBA-initiated CD34KO mice revealed that DMBA was metabolically activated into carcinogenic diol epoxides at both 200 and 400 nmol. Chronic exposure to TPA revealed that CD34KO skin developed and sustained epidermal hyperplasia. However, CD34KO hair follicles typically remained in telogen rather than transitioning into anagen growth, confirmed by retention of bromodeoxyuridine-labeled bulge stem cells within the hair follicle. Unique localization of the hair follicle progenitor cell marker MTS24 was found in interfollicular basal cells in TPA-treated WT mice, whereas staining remained restricted to the hair follicles of CD34KO mice, suggesting that progenitor cells migrate into epidermis differently between strains. These data show that CD34 is required for TPA-induced hair follicle stem cell activation and tumor formation in mice.

Published

2007

54. Expression profiling identifies smooth muscle cell diversity within human intima and plaque fibrous cap: loss of RGS5 distinguishes the cap.

Author

Adams LD, Geary RL, Li J, Rossini A, and Schwartz SM

Subjects

Carotid Arteries pathology, Carotid Arteries physiology, Humans, Immunohistochemistry, Muscle, Smooth, Vascular pathology, Phenotype, RGS Proteins metabolism, Tunica Intima pathology, Tunica Intima physiology, Tunica Media pathology, Tunica Media physiology, Carotid Artery Diseases genetics, Carotid Artery Diseases pathology, Gene Expression Profiling, Muscle, Smooth, Vascular physiology, RGS Proteins genetics

Abstract

Background: The fibrous cap of the atherosclerotic lesion is believed to be critical to stability because disruption of the cap is the final event leading to plaque rupture. We have, therefore, used expression arrays to define the phenotype of the cap and other plaque components., Methods and Results: To identify unique expression programs able to distinguish the smooth muscle of the cap from other plaque smooth muscle cells, RNA profiles were determined in human carotid artery media, nonatherosclerotic adjacent intima, fibrous cap of advanced atherosclerotic plaques, and whole advanced plaque with cDNA arrays covering 21,000 or 26,000 Unigene clusters. The molecular signature of each tissue was dominated by a core gene-set with differential expression of <1% of clusters assayed., Conclusions: Both intima and cap expressed novel genes not previously associated with SMC pathology. If the cap is derived from a unique subpopulation, this pattern is the signature of that particular set of cells. The loss of RGS5 in the fibrous cap is of particular interest because of its role in vessel development and physiology.

Published

2006

55. Two-dimensional gel electrophoresis.

Author

Adams LD and Gallagher SR

Subjects

Electrophoresis, Gel, Two-Dimensional instrumentation, Electrophoresis, Polyacrylamide Gel instrumentation, Electrophoresis, Polyacrylamide Gel methods, Hydrogen-Ion Concentration, Isoelectric Focusing instrumentation, Isoelectric Focusing methods, Proteins chemistry, Electrophoresis, Gel, Two-Dimensional methods

Abstract

Two-dimensional gel electrophoresis is the combination of two high-resolution electrophoretic procedures (isoelectric focusing and SDS-polyacrylamide gel electrophoresis) to provide much greater resolution than either procedure alone. In the first-dimension gel, solubilized proteins are separated according to their isoelectric point (pI) by isoelectric focusing. This gel is then applied to the top of an SDS-slab gel and electrophoresed. The proteins in the first-dimension gel migrate into the second-dimension gel where they are separated on the basis of their molecular weight. The basic protocols in this unit are based on the type of equipment originally described by O'Farrell in 1975. For very basic or very acidic proteins, two alternate protocols are provided. A third alternate protocol describes how two-dimensional electrophoresis can be performed using a minigel system. Protein sample preparation is presented in the support protocol.

Published

2005

56. Transplantation of embryonic stem cells overexpressing Bcl-2 promotes functional recovery after transient cerebral ischemia.

Author

Wei L, Cui L, Snider BJ, Rivkin M, Yu SS, Lee CS, Adams LD, Gottlieb DI, Johnson EM Jr, Yu SP, and Choi DW

Subjects

Animals, Cell Line, Ischemic Attack, Transient metabolism, Male, Mice, Proto-Oncogene Proteins c-bcl-2 physiology, Rats, Rats, Wistar, Stem Cells metabolism, Gene Expression Regulation, Developmental physiology, Ischemic Attack, Transient physiopathology, Ischemic Attack, Transient therapy, Proto-Oncogene Proteins c-bcl-2 biosynthesis, Proto-Oncogene Proteins c-bcl-2 genetics, Recovery of Function physiology, Stem Cell Transplantation methods

Abstract

The study tested the hypothesis that transplantation of embryonic stem (ES) cells into rat cortex after a severe focal ischemia would promote structural repair and functional recovery. Overexpression of the human anti-apoptotic gene bcl-2 in ES cells was tested for increasing survival and differentiation of transplanted cells and promoting functional benefits. Mouse ES cells, pretreated with retinoic acid to induce differentiation down neural lineages, were transplanted into the post-infarct brain cavity of adult rats 7 days after 2-h occlusion of the middle cerebral artery (MCA). Over 1-8 weeks after transplantation, the lesion cavity filled with ES cell-derived cells that expressed markers for neurons, astrocytes, oligodendrocytes, and endothelial cells. ES cell-derived neurons exhibited dendrite outgrowth and formed a neuropil. ES cell-transplanted animals exhibited enhanced functional recovery on neurological and behavioral tests, compared to control animals injected with adult mouse cortical cells or vehicle. Furthermore, transplantation with ES cells overexpressing Bcl-2 further increased the survival of transplanted ES cells, neuronal differentiation, and functional outcome. This study supports that ES cell transplantation and gene modification may have values for enhancing recovery after stroke.

Published

2005

57. Regulator of G protein signaling 5 marks peripheral arterial smooth muscle cells and is downregulated in atherosclerotic plaque.

Author

Li J, Adams LD, Wang X, Pabon L, Schwartz SM, Sane DC, and Geary RL

Subjects

Animals, Brain blood supply, Brain metabolism, Down-Regulation, Intestine, Small blood supply, Intestine, Small metabolism, Kidney blood supply, Kidney metabolism, Macaca fascicularis, Myocardium metabolism, RGS Proteins genetics, RNA, Messenger genetics, Arteriosclerosis metabolism, Blood Vessels metabolism, Myocytes, Smooth Muscle metabolism, RGS Proteins metabolism

Abstract

Objective: Regulator of G protein signaling 5 (RGS5), an inhibitor of Galpha(q) and Galpha(i) activation, was recently identified among genes highly expressed in smooth muscle cells (SMCs) of aorta but not vena cava. This finding prompted the hypothesis that RGS5 provides long-term G protein inhibition specific to normal arterial SMC populations and that loss of expression may in turn contribute to arterial disease., Methods: To test this hypothesis we characterized RGS5 gene expression throughout the vasculature of nonhuman primates to determine whether RGS5 was restricted to arteries in other vascular beds and whether expression was altered in arterial disease., Results: In situ hybridization localized RGS5 message to medial SMCs of peripheral arteries, including carotid, iliac, mammary, and renal arteries, but not accompanying veins. SMCs of many small arteries and arterioles also expressed RGS5, including glomerular afferent arterioles critical to blood pressure regulation. Differential expression persisted in culture, inasmuch as RGS5 message was significantly higher in SMCs derived from arteries than from veins at real-time polymerase chain reaction. It was remarkable that the only major arterial bed lacking RGS5 was the coronary circulation. In atherosclerotic peripheral arteries RGS5 was expressed in medial SMCs, but was sharply downregulated in plaque SMCs., Conclusion: These data identify RGS5 as a new member of a short list of genes uniquely expressed in peripheral arteries but not coronary arteries. Persistence of an arterial pattern of RGS5 expression in culture and lack of expression in coronary arteries support a unique SMC phenotype fixed by distinct lineage or differentiation pathways. The association between loss of expression and arterial wall disease has prompted the new hypothesis that prolonged inhibition by RGS5 of vasoactive or trophic G protein signaling is critical to normal peripheral artery function.

Published

2004

58. Two-dimensional gel electrophoresis.

Author

Adams LD and Gallagher SR

Subjects

Electrophoresis, Gel, Two-Dimensional instrumentation, Electrophoresis, Polyacrylamide Gel instrumentation, Electrophoresis, Polyacrylamide Gel methods, Isoelectric Focusing instrumentation, Isoelectric Focusing methods, Isoelectric Point, Molecular Weight, Electrophoresis, Gel, Two-Dimensional methods, Proteins analysis

Abstract

Two-dimensional gel electrophoresis is the combination of two high-resolution electrophoretic procedures (isoelectric focusing and SDS-polyacrylamide gel electrophoresis) to provide much greater resolution than either procedure alone. In the first-dimension gel, solubilized proteins are separated according to their isoelectric point (pI) by isoelectric focusing. This gel is then applied to the top of an SDS-slab gel and electrophoresed. The proteins in the first-dimension gel migrate into the second-dimension gel where they are separated on the basis of their molecular weight. The basic protocols in this unit are based on the type of equipment originally described by O'Farrell in 1975. For very basic or very acidic proteins, two alternate protocols are provided. A third alternate protocol describes how two-dimensional electrophoresis can be performed using a minigel system. Protein sample preparation is presented in the support protocol.

Published

2004

59. Cross-linking in the living cell locates the site of action of oxazolidinone antibiotics.

Author

Colca JR, McDonald WG, Waldon DJ, Thomasco LM, Gadwood RC, Lund ET, Cavey GS, Mathews WR, Adams LD, Cecil ET, Pearson JD, Bock JH, Mott JE, Shinabarger DL, Xiong L, and Mankin AS

Subjects

Amino Acid Sequence, Binding Sites, Electrophoresis, Polyacrylamide Gel, Models, Chemical, Models, Genetic, Models, Molecular, Molecular Sequence Data, Nucleic Acid Conformation, Peptides chemistry, Protein Binding, Protein Conformation, Protein Structure, Tertiary, RNA metabolism, RNA, Ribosomal, 23S metabolism, RNA, Transfer metabolism, Staphylococcus aureus metabolism, Transcription Factors chemistry, Anti-Bacterial Agents pharmacology, Cross-Linking Reagents pharmacology, Oxazolidinones pharmacology, Protein Synthesis Inhibitors pharmacology

Abstract

Oxazolidinone antibiotics, an important new class of synthetic antibacterials, inhibit protein synthesis by interfering with ribosomal function. The exact site and mechanism of oxazolidinone action has not been elucidated. Although genetic data pointed to the ribosomal peptidyltransferase as the primary site of drug action, some biochemical studies conducted in vitro suggested interaction with different regions of the ribosome. These inconsistent observations obtained in vivo and in vitro have complicated the understanding of oxazolidinone action. To localize the site of oxazolidinone action in the living cell, we have cross-linked a photoactive drug analog to its target in intact, actively growing Staphylococcus aureus. The oxazolidinone cross-linked specifically to 23 S rRNA, tRNA, and two polypeptides. The site of cross-linking to 23 S rRNA was mapped to the universally conserved A-2602. Polypeptides cross-linked were the ribosomal protein L27, whose N terminus may reach the peptidyltransferase center, and LepA, a protein homologous to translation factors. Only ribosome-associated LepA, but not free protein, was cross-linked, indicating that LepA was cross-linked by the ribosome-bound antibiotic. The evidence suggests that a specific oxazolidinone binding site is formed in the translating ribosome in the immediate vicinity of the peptidyltransferase center.

Published

2003

60. Software for pest-management science: computer models and databases from the United States Department of Agriculture-Agricultural Research Service.

Author

Wauchope RD, Ahuja LR, Arnold JG, Bingner R, Lowrance R, van Genuchten MT, and Adams LD

Subjects

Computer Simulation, Databases, Factual, Pesticides metabolism, United States, Agriculture methods, Pest Control methods, Research Design, Software, United States Department of Agriculture

Abstract

We present an overview of USDA Agricultural Research Service (ARS) computer models and databases related to pest-management science, emphasizing current developments in environmental risk assessment and management simulation models. The ARS has a unique national interdisciplinary team of researchers in surface and sub-surface hydrology, soil and plant science, systems analysis and pesticide science, who have networked to develop empirical and mechanistic computer models describing the behavior of pests, pest responses to controls and the environmental impact of pest-control methods. Historically, much of this work has been in support of production agriculture and in support of the conservation programs of our 'action agency' sister, the Natural Resources Conservation Service (formerly the Soil Conservation Service). Because we are a public agency, our software/database products are generally offered without cost, unless they are developed in cooperation with a private-sector cooperator. Because ARS is a basic and applied research organization, with development of new science as our highest priority, these products tend to be offered on an 'as-is' basis with limited user support except for cooperating R&D relationship with other scientists. However, rapid changes in the technology for information analysis and communication continually challenge our way of doing business.

Published

2003

61. Vascular failure: a hypothesis.

Author

Schwartz SM, Geary RL, and Adams LD

Subjects

Humans, Vascular Diseases therapy, Vascular Diseases genetics, Vascular Diseases physiopathology

Abstract

Although cardiac failure has been studied extensively, vascular failure is not a recognizable term. We suggest that it is reasonable to argue that failure of the vessel to control its mass, contractile capacity, and lumen will involve pathways similar to cardiac failure. Vascular failure, or perhaps more accurately arterial failure, has very different consequences. Failure to control mass and external diameter will result in hypertension or loss of lumen in atherosclerosis. We review what is known about this normal remodeling response and its failure, and propose directions for research.

Published

2003

62. Suppression subtractive hybridization identifies distinctive expression markers for coronary and internal mammary arteries.

Author

Qin M, Zeng Z, Zheng J, Shah PK, Schwartz SM, Adams LD, and Sharifi BG

Subjects

Animals, Arteriosclerosis genetics, Blotting, Northern, Cadherins analysis, Cadherins genetics, Caveolin 1, Caveolins analysis, Caveolins genetics, Claudins, DNA Probes, Immunoblotting, In Vitro Techniques, Membrane Proteins analysis, Membrane Proteins genetics, Reference Values, Ribonuclease, Pancreatic analysis, Ribonuclease, Pancreatic genetics, Swine, Tenascin analysis, Tenascin genetics, Coronary Vessels metabolism, DNA, Complementary analysis, Gene Expression, Mammary Arteries metabolism

Abstract

Objective: We sought to identify differentially expressed genes in the athero-prone coronary artery and athero-resistant internal mammary arteries., Methods and Results: Using suppressive subtraction hybridization, we generated reciprocal cDNA collections of representative mRNAs specific to porcine coronary arteries versus porcine mammary arteries. We screened 1000 suppressive subtraction hybridization cDNA clones by dot blot array and sequenced 600 of those showing the most marked expression differences. Northern blot, in situ hybridization, and immunostaining confirmed the differential gene expression patterns identified by the dot blot arrays. Genes associated with mammary arteries included claudin-10 and h-cadherin, which are genes associated with tight junctions and intermediate junctions. In contrast, genes associated with proatherosclerotic processes, such as lipid retention and metabolism, inflammation, and cell growth, were preferentially expressed in coronary arteries., Conclusions: Normal coronary arteries have gene expression program that is significantly different than internal mammary arteries. These differences may partly explain the resistance of coronary arteries and internal mammary arteries to atherosclerosis.

Published

2003

63. Double lox targeting for neural cell transgenesis.

Author

Adams LD, Choi L, Xian HQ, Yang A, Sauer B, Wei L, and Gottlieb DI

Subjects

Animals, Cell Differentiation genetics, Cells, Cultured, Male, Models, Biological, Mutagenesis, Insertional methods, Neurons cytology, Rats, Rats, Wistar, Receptors, Oxidized LDL, Scavenger Receptors, Class E, Stem Cells cytology, Transgenes genetics, Cell Culture Techniques methods, Gene Targeting methods, Neurons metabolism, Receptors, LDL genetics, Stem Cell Transplantation methods, Stem Cells metabolism

Abstract

ES cells differentiated along the neural lineage in vitro are an attractive model system. Here we have developed ES cell lines that are suitable for inserting transgenes at a single chromosomal site. ES cell line CE1 (for Cassette Exchange) contains one "acceptor" module (CE1) that allows for efficient double lox targeting. The site is also permissive for gene expression in neural progenitor cells, as well as differentiated neurons and glia. Line CE2 was derived by swapping a puromycin resistance cassette into CE1. Neural progenitors derived from this line are puromycin-resistant. A beta-actin/GFP expression cassette was inserted into the CE1 site to create CE3. The CE3 cell line was differentiated into neural cells and displayed strong EGFP expression in neural progenitors, differentiated neurons and glia. Differentiated CE3 ES cells (4-/4+ RA) were transplanted into the injured rat somatosensory cortex where many of the transplanted cells survived and differentiated into neurons expressing GFP. This strategy for creating sets of transgenic lines with multiple cassettes inserted into a single chromosomal site provides a powerful tool for studying development and function of ES cell-derived neural cells. Many of these will be useful in transplantation research.

Published

2003

64. Expression profiling identifies 147 genes contributing to a unique primate neointimal smooth muscle cell phenotype.

Author

Geary RL, Wong JM, Rossini A, Schwartz SM, and Adams LD

Subjects

Animals, Aorta chemistry, Aorta metabolism, Aorta transplantation, Blotting, Northern methods, Chondroitin Sulfate Proteoglycans genetics, Collagen Type I genetics, Gene Expression Profiling statistics & numerical data, Iliac Artery chemistry, Iliac Artery metabolism, In Situ Hybridization methods, Lectins, C-Type, Macaca fascicularis, Muscle, Smooth, Vascular cytology, Myosin Heavy Chains genetics, Oligonucleotide Array Sequence Analysis statistics & numerical data, Phenotype, RGS Proteins genetics, RNA, Ribosomal, 28S genetics, Venae Cavae chemistry, Venae Cavae metabolism, Venae Cavae transplantation, Versicans, Gene Expression Profiling methods, Genes genetics, Muscle, Smooth, Vascular chemistry, Muscle, Smooth, Vascular metabolism, Oligonucleotide Array Sequence Analysis methods, Tunica Intima chemistry, Tunica Intima metabolism

Abstract

Objective: This study represents the first in an effort to systematically characterize different intimas by using expression array analysis., Methods and Results: We compared smooth muscle cells (SMCs) of the neointima formed 4 weeks after aortic grafting with those from normal aorta and vena cava from cynomolgus monkeys. Hybridization to cDNA arrays identified subsets of 147 and 45 genes differentially expressed in the neointima versus the aorta and vena cava, respectively. The expression pattern differentiating neointima from aortic SMCs was characterized largely by suppression. Only 13 genes were induced in the neointima: 7 encoded matrix proteins (6 collagens and 1 versican) and 2 encoded inducers of matrix synthesis (osteoblast-specific factor-2/Cbfa1 and connective tissue growth factor). The genes suppressed most in the neointima included the regulator of G-protein signaling-5, SPARClike-1/hevin, and nonmuscle myosin heavy chain-B. A smaller gene set differentiated the neointima from the vena cava. Most were induced (39 of 45 genes), and overlap with the neointima-aorta set was significant (10 of 13 genes). Array results were validated with Northern analysis, in situ hybridization, or immunohistochemistry., Conclusions: These data underscore the importance of matrix synthesis in neointimal maturation, and novel genes, newly associated with neointimal SMCs (regulator of G-protein signaling-5 and osteoblast-specific factor-2/Cbfa1), have raised new hypotheses regarding the pathogenesis of intimal hyperplasia.

Published

2002

65. Open-label randomized trial of torsemide compared with furosemide therapy for patients with heart failure.

Author

Murray MD, Deer MM, Ferguson JA, Dexter PR, Bennett SJ, Perkins SM, Smith FE, Lane KA, Adams LD, Tierney WM, and Brater DC

Subjects

Aged, Biological Availability, Diuretics pharmacokinetics, Female, Furosemide pharmacokinetics, Hospitalization, Humans, Male, Middle Aged, Quality of Life, Sulfonamides pharmacokinetics, Torsemide, Treatment Outcome, Diuretics therapeutic use, Furosemide therapeutic use, Heart Failure drug therapy, Sulfonamides therapeutic use

Abstract

Purpose: Because the bioavailability of oral furosemide is erratic and often incomplete, we tested the hypothesis that patients with heart failure who were treated with torsemide, a predictably absorbed diuretic, would have more favorable clinical outcomes than would those treated with furosemide., Patients and Methods: We conducted an open-label trial of 234 patients with chronic heart failure (mean [+/- SD] age, 64 +/- 11 years) from an urban public health care system. Patients received oral torsemide (n = 113) or furosemide (n = 121) for 1 year. The primary endpoint was readmission to the hospital for heart failure. Secondary endpoints included readmission for all cardiovascular causes and for all causes, numbers of hospital days, and health-related quality of life., Results: Compared with furosemide-treated patients, torsemide-treated patients were less likely to need readmission for heart failure (39 [32%] vs. 19 [17%], P <0.01) or for all cardiovascular causes (71 [59%] vs. 50 [44%], P = 0.03). There was no difference in the rate of admissions for all causes (92 [76%] vs. 80 [71%], P = 0.36). Patients treated with torsemide had significantly fewer hospital days for heart failure (106 vs. 296 days, P = 0.02). Improvements in dyspnea and fatigue scores from baseline were greater among patients treated with torsemide, but the differences were statistically significant only for fatigue scores at months 2, 8, and 12., Conclusions: Compared with furosemide-treated patients, torsemide-treated patients were less likely to be readmitted for heart failure and for all cardiovascular causes, and were less fatigued. If our results are confirmed by blinded trials, torsemide may be the preferred loop diuretic for patients with chronic heart failure.

Published

2001

66. Two-dimensional gel electrophoresis using the ISO-DALT system.

Author

Adams LD

Subjects

Animals, Electrophoresis, Gel, Two-Dimensional methods, Equipment Design, Humans, Molecular Weight, Proteins chemistry, Electrophoresis, Gel, Two-Dimensional instrumentation, Electrophoresis, Polyacrylamide Gel instrumentation, Isoelectric Focusing instrumentation, Proteins isolation & purification

Abstract

Two high-resolution electrophoretic procedures (isoelectric focusing and SDS-polyacrylamide gel electrophoresis) are combined in this unit to provide much greater resolution than either of the individual procedures. Solubilized proteins are first separated according to their isoelectric point by isoelectric focusing in a tube gel. This first dimension gel is then applied to the top of an SDS-polyacrylamide slab gel and electrophoresed. The proteins in the first-dimension gel migrate into the second-dimension gel where they are further separated on the basis of their molecular size. The ISO-DALT system was specifically designed for running multiple high-resolution two-dimensional gels at one time.

Published

2001

67. A comparison of aorta and vena cava medial message expression by cDNA array analysis identifies a set of 68 consistently differentially expressed genes, all in aortic media.

Author

Adams LD, Geary RL, McManus B, and Schwartz SM

Subjects

Adult, Animals, Blotting, Northern, Culture Media, DNA Probes, DNA, Complementary analysis, Female, Humans, In Situ Hybridization, Macaca, Male, Middle Aged, Oligonucleotide Array Sequence Analysis, RGS Proteins genetics, Rats, Rats, Sprague-Dawley, Aorta physiology, Gene Expression Regulation, Venae Cavae physiology

Abstract

We performed a systematic analysis of gene expression in arteries and veins by comparing message profiles of macaque aorta and vena cava media using a cDNA array containing 4048 known human genes, approximately 35% of currently named human genes (approximately 11,000). The data show extensive differences in RNA expression in artery versus vein media. Sixty-eight genes had consistent elevation in message expression by the aorta, but none were elevated in the vena cava. The most differentially expressed gene was regulator of G-protein signaling (RGS) 5, at an expression ratio of 46.5+/-12.6 (mean+/-SEM). The data set also contained 2 genes already known to be expressed in the aorta, elastin at 5.0+/-1.4, and the aortic preferentially expressed gene 1 (APEG-1) at 2.3+/-0.6. We chose to analyze RGS5 expression further because of its high level of differential expression in the aorta. Levels of RGS5 mRNA were confirmed by Northern analysis and in situ hybridization. A human tissue RNA dot blot showed that RGS5 message is highest in aorta, followed by small intestine, stomach, and then heart. Northern analysis confirmed that RGS5 expression in human aorta is higher than in any region of the heart. RGS5 is a G-protein signaling regulator of unknown specificity most homologous to RGS4, an inhibitory regulator of pressure-induced cardiac hypertrophy. The expression pattern of the 68 differential genes as a whole is a start toward identifying the molecular phenotypes of arteries and veins on a systematic basis.

Published

2000

68. Fas/FADD-mediated activation of a specific program of inflammatory gene expression in vascular smooth muscle cells.

Author

Schaub FJ, Han DK, Liles WC, Adams LD, Coats SA, Ramachandran RK, Seifert RA, Schwartz SM, and Bowen-Pope DF

Subjects

Animals, Carotid Arteries immunology, Carotid Arteries pathology, Caspases metabolism, Chemokine CCL2 biosynthesis, Fas-Associated Death Domain Protein, Gene Expression Regulation, Humans, Interleukin-1 metabolism, Interleukin-8 biosynthesis, Rats, Rats, Inbred F344, Up-Regulation, Adaptor Proteins, Signal Transducing, Apoptosis, Carrier Proteins metabolism, Inflammation genetics, Muscle, Smooth, Vascular immunology, fas Receptor metabolism

Abstract

Apoptosis of smooth muscle cells is a common feature of vascular lesions but its pathophysiological significance is not known. We demonstrate that signals initiated by regulated Fas-associated death domain protein overexpression in rat vascular smooth muscle cells in the carotid artery induce expression of monocyte-chemoattractant protein-1 and interleukin-8, and cause massive immigration of macrophages in vivo. These chemokines, and a specific set of other pro-inflammatory genes, are also upregulated in human vascular smooth muscle cells during Fas-induced apoptosis, in part through a process that requires interleukin-1alpha activation. Induction of a pro-inflammatory program by apoptotic vascular smooth muscle cells may thus contribute to the pathogenesis of vascular disease.

Published

2000

69. CART peptides.

Author

Kuhar MJ, Adams LD, Hunter RG, Vechia SD, and Smith Y

Subjects

Amino Acid Sequence, Animals, Feeding Behavior, Humans, Molecular Sequence Data, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Neurotransmitter Agents genetics, Neurotransmitter Agents metabolism, RNA, Messenger, Nerve Tissue Proteins physiology, Neurotransmitter Agents physiology

Abstract

CART peptides are among the newest putative peptide neurotransmitter/cotransmitters. They show no significant homology to any other peptide, and they are thought to have a role in reward and reinforcement, feeding, development, sensory processing, stress and endocrine control.

Published

2000

70. CART: from gene to function.

Author

Adams LD, Gong W, Vechia SD, Hunter RG, and Kuhar MJ

Subjects

Animals, Mice, Nerve Tissue Proteins genetics

Abstract

CART was identified as a novel mRNA regulated by psychostimulant drugs. CART peptides appear to be neurotransmitters involved in a variety of functions such as feeding. The mouse gene has been characterized and localized to Chromosome 13. The processing of CART peptides is evident in Western blotting studies.

Published

1999

71. A systematic analysis of 40 random genes in cultured vascular smooth muscle subtypes reveals a heterogeneity of gene expression and identifies the tight junction gene zonula occludens 2 as a marker of epithelioid "pup" smooth muscle cells and a participant in carotid neointimal formation.

Author

Adams LD, Lemire JM, and Schwartz SM

Subjects

Age Factors, Angioplasty, Balloon adverse effects, Animals, Aorta cytology, Aorta injuries, Aorta physiology, Biomarkers, Blotting, Northern, Carotid Arteries chemistry, Carotid Arteries growth & development, Carotid Artery Injuries pathology, Carotid Artery Injuries physiopathology, Cells, Cultured, DNA, Complementary isolation & purification, Gene Library, Male, Membrane Proteins analysis, Muscle, Smooth, Vascular cytology, Muscle, Smooth, Vascular injuries, Phenotype, Phosphoproteins analysis, Phosphoproteins genetics, RNA, Messenger analysis, Rats, Rats, Inbred WKY, Tight Junctions chemistry, Tunica Intima chemistry, Tunica Intima cytology, Tunica Intima growth & development, Tunica Media chemistry, Tunica Media cytology, Tunica Media physiology, Zonula Occludens-1 Protein, Zonula Occludens-2 Protein, Carotid Arteries cytology, Gene Expression Regulation, Developmental, Membrane Proteins genetics, Muscle, Smooth, Vascular physiology, Tight Junctions genetics

Abstract

An accumulation of evidence suggests that vascular smooth muscle is composed of cell subpopulations with distinct patterns of gene expression. Much of this evidence has come from serendipitous discoveries of genes marking phenotypically distinct aortic cultures derived from 12-day-old and 3-month-old rats. To identify more systematic differences, we isolated 40 genes at random from libraries of these 2 cultures and examined message expression patterns. To determine consistency of differential expression, we measured mRNA levels in 4 sets of cultures in 6 phenotypically distinct aortic cell clones and in balloon injured rat carotid arteries to determine the relevance of these differences in vitro to in vivo biology. The following 5 consistently differentially expressed genes were identified in vitro: zonula occludens 2 (ZO-2); peroxisome proliferator-activated receptor delta (PPARdelta); secreted protein, acidic and rich in cysteine (SPARC); alpha1(I)collagen; and A2, an uncharacterized gene. We examined these 5 clones during carotid artery injury and an inconsistently differentially expressed clone Krox-24 because, as an early response transcription factor, it could be involved in the injury response. PPARdelta, A2, and Krox-24 mRNAs were upregulated during the day after injury. ZO-2 and alpha1(I)collagen messages were modulated for up to a month, whereas SPARC message showed no consistent change. An analysis of ZO-2 and other tight junction genes indicates that tight junctions may play a role in smooth muscle biology. These data suggest that a systematic analysis of these libraries is likely to identify a very large number of differentially expressed genes. ZO-2 is particularly intriguing both because of this tight junction gene's pattern of prolonged over-expression after injury and because of its potential role in determining the distinctive epithelioid phenotype of smooth muscle cells identified in rat and other species.

Published

1999

72. In vitro metabolism of ceftiofur in bovine tissues.

Author

Olson SC, Beconi-Barker MG, Smith EB, Martin RA, Vidmar TJ, and Adams LD

Subjects

Animals, Cattle, Cephalosporins analysis, Cephalosporins chemistry, Cystine pharmacology, Glutathione pharmacology, In Vitro Techniques, Male, Microsomes, Liver metabolism, Subcellular Fractions metabolism, Time Factors, Cephalosporins metabolism, Kidney metabolism, Liver metabolism, Lung metabolism, Muscles metabolism

Abstract

The metabolism of ceftiofur in bovine kidney, liver, muscle and lung, and the effects of the presence of cystine and glutathione in the media were evaluated using S-9 and microsomal tissue fractions. Conversion of ceftiofur to desfuroylceftiofur (DFC) was catalyzed by an esterase which was most active in kidney, followed by liver. It was not very active in muscle and lung. After DFC was liberated, it rapidly bound primarily to tissue proteins (> 56%), and was also conjugated to cysteine and glutathione. Production of DFC-cysteine by disulfide exchange of DFC with cystine and production of DFC-glutathione by conjugation of DFC to glutathione occurred in buffer if glutathione and cystine were present in the medium. These conjugations were also observed in incubations with tissue fractions, indicating that they were not inhibited by the tissues endogenous molecules. In addition, the metabolism of DFC-glutathione to DFC-cysteine was observed when tissue proteins were present. The metabolism of DFC-glutathione to DFC-cysteine was faster in kidney than in liver. Metabolites devoid of an intact beta-lactam ring were not observed in these in vitro studies.

Published

1998

73. Heterophilic NCAM-mediated cell adhesion to proteoglycans from chick embryonic brain membranes.

Author

Storms SD, Anvekar VM, Adams LD, and Murray BA

Subjects

Animals, Brain embryology, Cell Fractionation, Chick Embryo, Chondroitin Lyases, Chondroitin Sulfate Proteoglycans metabolism, Chromatography, Ion Exchange, Glycosaminoglycans pharmacology, Heparan Sulfate Proteoglycans, Heparin Lyase, Heparitin Sulfate metabolism, L Cells, Ligands, Mice, Neural Cell Adhesion Molecules isolation & purification, Octoxynol, Polysaccharide-Lyases, Transfection, Brain cytology, Cell Adhesion physiology, Cell Membrane metabolism, Neural Cell Adhesion Molecules metabolism, Proteoglycans metabolism

Abstract

The vertebrate neural cell adhesion molecule NCAM mediates adhesion by both homophilic and heterophilic mechanisms, with heparan sulfate proteoglycans (HSPGs) being likely heterophilic ligands. In this study, transfected chicken NCAM polypeptides expressed on mouse L cells mediated the adhesion of these cells to several different heparan sulfate proteoglycans in nonionic detergent extracts of Embryonic Day 10 chicken brain membranes. In addition, adhesion inhibition experiments suggested a hitherto-undetected role for chondroitin sulfate proteoglycans in the stimulation of NCAM-mediated adhesion to some, but not all, of the HSPG ligands. Our experiments support the view that NCAM is a multivalent adhesive molecule whose function is affected by interactions with extracellular matrix and cell surface molecules.

Published

1996

74. The large cytoplasmic domain is not required for concentration of N-CAM at cell-cell contacts in transfected mouse neuroblastoma cells.

Author

Woo MK, Kil SH, Adams LD, Nguyen TN, and Murray BA

Subjects

Animals, Cell Adhesion Molecules, Neuronal metabolism, Chickens, Cytoplasm ultrastructure, Fluorescent Antibody Technique, In Vitro Techniques, Mice, Neuroblastoma, Structure-Activity Relationship, Transfection, Tumor Cells, Cultured, Cell Adhesion, Cell Adhesion Molecules, Neuronal chemistry

Abstract

We examined the localization of the 140- and 180-kDa transmembrane isoforms of chicken N-CAM following transfection into mouse N2A neuroblastoma cells. Both isoforms were expressed at the cell surface and became partially or completely localized at areas of cell-cell contact after several days of culture or of in vitro differentiation. These results indicate that the presence of the large cytoplasmic domain of the 180-kDa N-CAM isoform is not necessary to bring about the localization of N-CAM to points of cell-cell contact.

Published

1993

75. Tissue distribution and cellular localization of hsp56, an FK506-binding protein. Characterization using a highly specific polyclonal antibody.

Author

Ruff VA, Yem AW, Munns PL, Adams LD, Reardon IM, Deibel MR Jr, and Leach KL

Subjects

Animals, Antibodies immunology, Antibody Specificity, Carrier Proteins immunology, Cells, Cultured, Electrophoresis, Gel, Two-Dimensional, Fluorescent Antibody Technique, Heat-Shock Proteins immunology, Humans, Male, Rats, Rats, Sprague-Dawley, Tacrolimus Binding Proteins, Tissue Distribution, Carrier Proteins metabolism, Heat-Shock Proteins metabolism, Tacrolimus metabolism

Abstract

Heat shock protein 56 (hsp56) has been shown to be involved in two cellular pathways, as an immunophilin for FK506 and as a component of steroid receptor complexes. To help define its role in these cellular pathways, we have developed UPJ56, a polyclonal antibody raised against hsp56 purified from Jurkat cells. In Western blot experiments, hsp56 was highly expressed in rat thymus, liver, and spleen, with low levels in lung and muscle. In immunofluorescence experiments using untreated LLC-PK1 cells, fibrillar staining was seen in the cytoplasm, suggesting a cytoskeletal localization of hsp56. The nuclei were brightly stained, except for the nucleoli. Confocal microscopy demonstrated that the staining was present in all planes of the nucleus. These results suggest that hsp56 is expressed in tissues enriched in steroid receptors and is highly expressed in tissues involved in T cell function. Furthermore, the localization of hsp56 with the cytoskeleton and throughout the nucleus is consistent with its association with steroid receptor complexes.

Published

1992

76. Alpha-thrombin stimulates nuclear diglyceride levels and differential nuclear localization of protein kinase C isozymes in IIC9 cells.

Author

Leach KL, Ruff VA, Jarpe MB, Adams LD, Fabbro D, and Raben DM

Subjects

Animals, Cell Nucleus enzymology, Cell Nucleus metabolism, Cell Nucleus ultrastructure, Cells, Cultured, Cricetinae, Electrophoresis, Polyacrylamide Gel, Fluorescent Antibody Technique, Microscopy, Electron, Nuclear Proteins metabolism, Phosphorylation, Tetradecanoylphorbol Acetate pharmacology, Cell Nucleus drug effects, Diglycerides metabolism, Isoenzymes metabolism, Protein Kinase C metabolism, Thrombin pharmacology

Abstract

The mechanism by which an agonist, binding to a cell surface receptor, exerts an effect on events in the nucleus is not known. We have previously shown (Leach, K. L., Ruff, V. A., Wright, T. M., Pessin, M. S., and Raben, D. M. (1991) J. Biol. Chem. 266, 3215-3221) that alpha-thrombin treatment of IIC9 cells results in increased levels of cellular 1,2-diacylglycerol (DAG) and activation of protein kinase C (PKC). Here, we have examined whether changes in nuclear PKC and nuclear DAG also are induced following alpha-thrombin treatment. IIC9 cells were treated with 500 ng/ml alpha-thrombin, and nuclei were then isolated. Western blot analysis using isozyme-specific antibodies demonstrated the presence of PKC alpha, but not PKC epsilon or zeta in the nuclei of cells treated with either phorbol 12-myristate 13-acetate or alpha-thrombin. The increase in nuclear PKC alpha levels was accompanied by a 10-fold increase in nuclear PKC specific activity and stimulated phosphorylation of at least six nuclear proteins. The rise in nuclear PKC levels occurred rapidly and reached a maximum at 30-60 s, which was followed by a decline back to the control level over the next 15 min. In addition, alpha-thrombin treatment resulted in an immediate rise in DAG mass levels in the nuclear fractions. Kinetic analysis indicated that a maximum increase in DAG levels occurred 2.5-5 min after the addition of alpha-thrombin and remained elevated for at least 30 min. In cells labeled with [3H]myristic acid, alpha-thrombin treatment induced an increase in radiolabeled nuclear diglycerides, suggesting that the stimulated nuclear DAGs are derived, at least in part, from phosphatidylcholine. Our results suggest that increases in both nuclear DAG levels and PKC activity following alpha-thrombin treatment may play a role in mediating thrombin-induced nuclear responses such as changes in gene expression and cellular proliferation.

Published

1992

77. HIV-1 protease cleaves actin during acute infection of human T-lymphocytes.

Author

Adams LD, Tomasselli AG, Robbins P, Moss B, and Heinrikson RL

Subjects

Cell Line, Electrophoresis, Gel, Two-Dimensional, HIV-1 physiology, Humans, Hydrolysis, T-Lymphocytes microbiology, Actins metabolism, HIV Protease metabolism, HIV-1 enzymology

Abstract

Actin, one of the most abundant proteins of the cell, is hydrolyzed by the human immunodeficiency virus type 1 (HIV-1) protease during acute infection of cultured human T lymphocytes. The actin fragments produced during the course of infection are identical to those obtained by recombinant HIV-1 protease digests of (1) a lysate from uninfected T lymphocytes and (2) globular actin itself. Hydrolysis by the HIV-1 protease of physiologically important host cellular proteins during infection may have important consequences relative to viral pathogenesis.

Published

1992

78. Tumor progression- and metastasis-associated proteins identified using a model of locally recurrent rat mammary adenocarcinomas.

Author

Welch DR, McClure SA, Aeed PA, Bahner MJ, and Adams LD

Subjects

Amino Acids analysis, Animals, Electrophoresis, Polyacrylamide Gel, Female, Glycoproteins analysis, Lactoperoxidase analysis, Molecular Weight, Neoplasm Proteins chemistry, Rats, Rats, Inbred F344, Wheat Germ Agglutinins metabolism, Adenocarcinoma chemistry, Mammary Neoplasms, Experimental chemistry, Neoplasm Metastasis, Neoplasm Proteins analysis, Neoplasm Recurrence, Local chemistry

Abstract

A recently established model for local breast cancer recurrence using the 13762NF rat mammary adenocarcinoma was used to evaluate biologic and biochemical properties related to clinical outcome for this class of tumors. Sublines isolated from local tumor regrowths following surgical resection differed from each other and from the 'parental' cell lines for multiple phenotypes, including metastatic propensity. Local recurrence- and primary tumor-derived sublines were examined by two-dimensional polyacrylamide gel electrophoresis (2D-PAGE), lectin binding to electrophoretically separated proteins, and lactoperoxidase-catalyzed cell surface iodination; and differential protein patterns were compared to tumor progression and metastatic potential. 2D-PAGE revealed several quantitatively different spots which correlated with lung colonization potential. In particular, quantities of an apparently unique, non-cell-surface protein, P50.9 (Mr approximately 50,900, pI approximately 7.3) correlated inversely with metastatic propensity, suggesting that it may be associated with, among other possibilities, the negative regulation of the metastatic phenotype. P50.9 was unrelated to four similarly sized metastasis-associated proteins--tumor autocrine motility factor; the rat analog of tumor suppressor, p53; rat cytokeratin 14 or procathepsin D--as determined by amino acid analysis. A major wheat germ agglutinin binding sialoglycoprotein, gp93 (Mr approximately 93,000), was present in smaller amounts as cells were passaged in vivo and re-established as in vitro cultures [MTF7 greater than 'primary' tumor-derived lines (sc1, sc3) much greater than local recurrence-derived lines (LR1, LR1a, LR3, LR4, LR5, LR6)]. Besides cell surface glycoprotein losses, two of six local recurrence-derived sublines expressed a wheat germ agglutinin-binding sialoglycoprotein, gp110 (Mr approximately 110,000), previously undetected on any of the other cell lines including the parental populations. gp110 was found in LR3 and LR6 which were relatively highly metastatic; however, correlation with metastatic potential failed because gp110 was not present on the metastatic parental cell line, MTF7. These results demonstrate specific quantitative and qualitative protein differences associated with the selection of locally recurrent mammary tumors.

Published

1990

79. Effects of trospectomycin on serum sensitivity of Escherichia coli UC 9451.

Author

Cialdella JI, Ulrich RG, Liggett WF, Adams LD, and Marshall VP

Subjects

Bacterial Outer Membrane Proteins metabolism, Cell Membrane drug effects, Cell Membrane ultrastructure, Complement Pathway, Alternative drug effects, Complement Pathway, Classical drug effects, Electrophoresis, Polyacrylamide Gel, Gentamicins pharmacology, Humans, Microbial Sensitivity Tests, Microscopy, Electron, Spectinomycin pharmacology, Anti-Bacterial Agents pharmacology, Blood Bactericidal Activity drug effects, Escherichia coli drug effects, Spectinomycin analogs & derivatives

Abstract

Trospectomycin sulfate, a chemically synthesized analog of spectinomycin, exhibits a broad range of activity against both aerobes and anaerobes, including the etiological agents of sexually transmitted diseases. Its activity in vitro against Escherichia coli is considered only moderate. At subinhibitory levels, however, trospectomycin induced changes in a pathogenic strain of E. coli, UC 9451, which significantly increased its sensitivity to serum lysis. This strain of E. coli shows high-level resistance to serum in vitro, typically growing twofold within a 45-min incubation period. Following exposure to one-fifth the MIC of trospectomycin, greater than 99% of the bacteria were killed in 25% serum within 15 min. Surviving bacteria were static in this level of serum for over 3 h. Killing was due to lysis mediated by both the classical and alternative complement pathways. The bacteria exposed to trospectomycin were enlarged in both diameter and length, but they still grew at rates comparable to those of untreated bacteria. No other visible morphological changes could be directly related to the increase in serum sensitivity. The profile of outer membrane proteins obtained by sodium dodecyl sulfate-polyacrylamide gel electrophoresis was identical for trospectomycin-treated or untreated bacteria. However, the relative proportion of four major outer membrane proteins varied considerably.

Published

1990

80. Detection and recovery of proteins from gels following zinc chloride staining.

Author

Adams LD and Weaver KM

Subjects

Animals, Copper, Diffusion, Liver, Mice, Mice, Inbred BALB C, Potassium Chloride, Rats, Rosaniline Dyes, Chlorides, Electrophoresis, Polyacrylamide Gel, Proteins chemistry, Staining and Labeling, Zinc, Zinc Compounds

Abstract

This report describes a method for detecting proteins in SDS polyacrylamide gels using ZnCl2 and their recovery using passive elution. Washing unfixed gels in a dilute solution of ZnCl2 produces two desirable effects. First, it makes the proteins easily visible as clear zones in a white background, and second, it prevents loss of proteins due to diffusion into the wash solution. Compared to other commonly used methods of protein detection such as Coomassie, KCl, copper or silver staining, the zinc stain offers some distinct advantages. Zinc staining can be completed in 15 min for most applications, making it much faster than Coomassie or most silver stains. The zinc stain is more sensitive than Coomassie, KCl or copper stain. Since no harsh chemical conditions are used in the zinc staining procedure, recovery of proteins from the gel is facilitated. More than 90% of selected proteins were recovered from 2-D gels by simple elution from the gel pieces with a buffer containing 10 mM EDTA.

Published

1990

81. Rapid modulation of a 64 K dalton fibroblast protein: a PDGF mediated early cellular event.

Author

Singh JP, Bonin PD, and Adams LD

Subjects

Animals, Cell Line, Culture Media analysis, DNA biosynthesis, Electrophoresis, Gel, Two-Dimensional, Fibroblasts physiology, Gene Expression Regulation, Kinetics, Mice, Mice, Inbred BALB C, Molecular Weight, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins c-fos, Transcription, Genetic drug effects, Fibroblasts metabolism, Platelet-Derived Growth Factor pharmacology

Abstract

The results presented here reveal a novel platelet derived growth factor (PDGF) mediated early cellular event. Treatment of growth arrested Balb/c3T3 fibroblasts with PDGF induces a specific and rapid modulation of a 64,000 Dalton (64 KD) protein preexisting in quiescent cells. The kinetics of 64 KD protein modulation indicate that, temporally, this PDGF mediated step lies between the membrane associated immediate events such as receptor autophosphorylation or ion mobilization and the earliest known transcriptional event, the activation of the proto-oncogene c-fos.

Published

1989

82. Measuring various drug use dimensions with a calendar method.

Author

Adams LD and Henley JR Jr

Subjects

Humans, Time Factors, Substance-Related Disorders

Abstract

This note presents a technique used to acquire a variety of time-specific data on drug use. The calendar technique involves self-reported patterns of consumption and any changes therein, including cessation. Advantages of this technique over other approaches are discussed, and examples of the variety of use measures that can be derived from the calendar method are illustrated.

Published

1977

83. The antigenic relatedness of proteins from human and simian prostate fluid.

Author

Carter DB, Timmins JG, Adams LD, Lewis RW, Karr JP, Resnick MI, and Buhl AE

Subjects

Animals, Autoradiography, Body Fluids immunology, Electrophoresis, Humans, Macaca mulatta, Male, Molecular Weight, Prospective Studies, Species Specificity, Carrier Proteins immunology, Epitopes, Prostate metabolism, Prostatic Secretory Proteins

Abstract

Two-dimensional electrophoretic analysis of human prostate fluid reveals an abundant protein migrating to a molecular weight of 15 kD and an isoelectric point of 5.5. Polyclonal antibodies were raised specifically to microgram quantities of electrophoresed, excised, and eluted PSP15 (prostate secretory protein). Western immunoblot analysis using these antibodies showed they not only react to PSP15, but cross-react with simian prostate and human seminal fluid proteins of similar molecular weights. Two-dimensional gel immunoblots strongly suggest that the seminal protein and PSP15 are the same, thereby providing a more accessible source of the protein. The antibody to the human PSP15 cross-reacted with neither prostate fluid from the ventral lobe of the rat prostate nor the prostate fluid from the beagle dog.

Published

1985

84. Dietary management of canine and feline chronic renal failure.

Author

Polzin DJ, Osborne CA, Adams LD, and O'Brien TD

Subjects

Animal Nutritional Physiological Phenomena, Animals, Cats, Dogs, Kidney Failure, Chronic diet therapy, Cat Diseases diet therapy, Dog Diseases diet therapy, Kidney Failure, Chronic veterinary

Abstract

Nutritional therapy is the mainstay of management of chronic renal failure in dogs and cats. Diets designed for use in renal failure are typically reduced in protein, phosphorus, and sodium content. These and other dietary modifications are designed to prevent or ameliorate clinical signs of uremia, minimize disturbances associated with excesses or losses of electrolytes and minerals, arrest or retard progression of renal failure, and maintain adequate nutrition.

Published

1989

85. A nonurea electrophoretic gel system for resolution of polypeptides of Mr 2000 to Mr 200,000.

Author

DeWald DB, Adams LD, and Pearson JD

Subjects

Buffers, Electrophoresis, Polyacrylamide Gel, Isoelectric Focusing, Molecular Weight, Staining and Labeling, Urea, Peptides analysis, Proteins analysis

Abstract

A sodium dodecyl sulfate-polyacrylamide gel electrophoresis system which resolves proteins and peptides from Mr 2000 to Mr 200,000 is described. Gradients of polyacrylamide, crosslinker, and glycerol buffered in Tris-phosphate (pH 6.8) are employed. Neither urea nor a stacking gel is required. This system has been used to separate molecules below Mr 3000 which differed by only seven amino acid residues, yet has the capacity to survey masses up to Mr 200,000 on the same gel. Examples are given for separations of myoglobin cyanogen bromide fragments and adrenocorticotropin peptides. Utilizing the same gradient slab gel system in tandem with isoelectric focusing, a two-dimensional separation pattern of mammalian liver cell lysate is shown. A comparison of two different silver stain methods with this system is also given.

Published

1986

86. The lipolytic system in adipose tissue of Toronto-KK and C57BL/KsJ diabetic mice. Adenylate cyclase, phosphodiesterase and protein kinase activities.

Author

Kupiecki FP and Adams LD

Subjects

Adipose Tissue cytology, Animals, Diabetes Mellitus genetics, Disease Models, Animal, Epinephrine pharmacology, Male, Metabolism drug effects, Mice, Mice, Inbred C57BL, Phosphorus Radioisotopes, Tritium, Adenylyl Cyclases metabolism, Adipose Tissue enzymology, Diabetes Mellitus enzymology, Lipid Metabolism, Mice, Inbred Strains, Phosphoric Diester Hydrolases metabolism

Published

1974

87. Mode of fibroblast growth enhancement by human interleukin-1.

Author

Singh JP, Adams LD, and Bonin PD

Subjects

Animals, Cell Line, DNA biosynthesis, DNA drug effects, Fibroblasts cytology, Humans, Interphase, Platelet-Derived Growth Factor pharmacology, Cell Division, Interleukin-1 pharmacology

Abstract

Previous studies have demonstrated that interleukin-1 (IL-1) stimulates fibroblast growth (Schmidt, J. A., S. B. Mizel, D. Cohn, and I. Green. 1982. J. Immunol. 128:2177-2182) and binds to specific, high affinity receptors of BALB/c3T3 cells (Bird, T. A., and J. Saklatval. 1986. Nature (Lond.). 324:263-265, 266-268). We have investigated the mechanism of fibroblast growth stimulation by IL-1. Addition of fibroblast growth factor derived from platelets (PDGF) to a quiescent culture of BALB/c3T3 cells produced 8-10-fold increase in DNA synthesis during 24-h incubation. The cellular action of PDGF was mediated through competence induction and required synergistic action of plasma-derived factors for full mitogenic activity. When tested at a wide range of concentrations (0.1-100 pM), natural IL-1 or recombinant IL-1 produced only a maximum of 5-10% of DNA synthesis elicited in response to PDGF or serum. Induction of DNA synthesis required continuous presence of IL-1 and did not exhibit synergism with plasma. Competence induction and mitogenic stimulation by PDGF was associated with early induction of proteins P32, P38, P46-48, P75, and changes in cytoskeletal organization. Examination of these early cellular changes showed that IL-1 did not produce similar induction of cellular proteins and the morphological changes associated with growth stimulation. These results suggest that the mode of IL-1 action on BALB/c3T3 was not through competence induction. When IL-1 was added to cells rendered competent by brief exposure to PDGF, 10-15% additional DNA synthesis occurred during the first 24 h. Extended incubation of PDGF-treated cells in the presence of IL-1 revealed that the stimulation by IL-1 occurred predominantly during the subsequent cycle of DNA replication, wherein DNA synthesis reached three- to fivefold higher than the untreated cultures. We conclude (a) IL-1 alone is not a potent mitogen for BALB/c3T3 cells, and does not bring cells out of the growth arrest Go phase, (b) treatment with PDGF renders the cells more responsive to IL-1, (c) part of the IL-1 action on competent cells may be characterized as progression inducing activity, further, (d) our results indicate that action of IL-1 on PDGF-treated cells produces sustained DNA synthesis for an extended period, perhaps by preventing the entry of cells into growth arrest Go phase.

Published

1988

88. Increased amount of a 25-kilodalton phosphoprotein after v-mos transfection of CHO cells.

Author

Mayo JK, Sampson KE, Adams LD, Crumm ER, Kelly SL, and Abraham I

Subjects

Animals, Cell Line, Transformed, Oncogene Proteins v-mos, Phosphorylation, Protein Kinases genetics, Protein Kinases metabolism, Retroviridae Proteins genetics, Oncogenes, Phosphoproteins metabolism, Retroviridae Proteins metabolism, Transfection

Abstract

We transfected Chinese hamster ovary (CHO) cells with a cloned v-mos gene (pHT25). The mos family of oncogenes has previously been shown to have serine-threonine kinase activity. This kinase activity may be required for oncogenic transformation, although its exact biological role is unknown. We found that the transfected cells had an altered morphology, a slower doubling time, and an apparent increase in the amount of a 25-kilodalton (kDa) phosphoprotein that appeared to be of low abundance. Transfection of CHO cells with a cloned temperature-sensitive mos gene (ts159) led to isolation of a cell line that showed the presence of the 25-kDa phosphoprotein at the permissive but not at the nonpermissive temperature, suggesting a direct relationship between mos activity and the presence of this phosphoprotein. The characteristics of altered morphology and depressed growth rate were reminiscent of changes seen after the activation of the cyclic AMP-dependent protein kinase (PKA) in CHO cells. However, PKA activation did not stimulate phosphorylation of this 25-kDa protein, nor was there a change in total PKA activity in these cells. We suggest that the increased presence of the 25-kDa phosphoprotein is a consequence of the v-mos transfection and that it may be involved in the change of morphology and growth rate seen in the CHO cells. Phosphorylation of this protein may be a useful marker of mos and have some functional importance in the transformation of cells by the v-mos oncogene.

Published

1988

89. Alloxan-induced hyperglycemia in rats is reduced by 16,16-dimethyl-PGE2.

Author

Ruwart MJ, Sammons DW, Kolaja GJ, Rush BD, Friedle NM, and Adams LD

Subjects

Animals, Blood Glucose metabolism, Diabetes Mellitus, Experimental pathology, Female, Glucose Tolerance Test, Islets of Langerhans pathology, Rats, Rats, Inbred Strains, Time Factors, 16,16-Dimethylprostaglandin E2 therapeutic use, Diabetes Mellitus, Experimental drug therapy, Prostaglandins E, Synthetic therapeutic use

Abstract

Female rats were treated with subcutaneous 16,16-dimethyl-PGE2 (1-75 micrograms/kg) for 24, 18, and 0.5 h prior to and 6, 24, and 48 h after intravenous beta cell destruction. Protection was assessed by morphological examination of beta cells and the level of fasting hyperglycemia seen 72 h after alloxan treatment. Prostaglandin reduced the degree of alloxan-induced hyperglycemia in a dose-dependent fashion but had no demonstrable effect on morphological assessment of beta cell destruction. However, prostaglandin treatment by itself induced transient (0-2 h) hyperglycemia that could be correlated inversely with the level of fasting blood glucose observed 72 h after alloxan treatment. Administration of oral glucose, which mimics the prostaglandin-induced hyperglycemia, afforded protection against alloxan challenge comparable to that produced by the prostaglandin. Thus, it appears that reduction of alloxan-induced hyperglycemia by 16,16-dimethyl-PGE2 may be linked to the transient hyperglycemia produced prior to alloxan administration.

Published

1983

90. Insulin-induced rapid decrease of a major protein in fat cell plasma membranes.

Author

Schoenle EJ, Adams LD, and Sammons DW

Subjects

Adipose Tissue drug effects, Animals, Calcium pharmacology, Cell Membrane metabolism, Dose-Response Relationship, Drug, Egtazic Acid pharmacology, Lanthanum pharmacology, Male, Peptides pharmacology, Rats, Rats, Inbred Strains, Somatomedins pharmacology, Time Factors, Vanadates, Vanadium pharmacology, Adipose Tissue cytology, Insulin pharmacology, Membrane Proteins metabolism

Abstract

In order to increase our understanding of the mode of action of insulin in rat fat cells, we investigated the effect of insulin on protein concentrations in purified fat cell fractions using two-dimensional electrophoresis in combination with an ultrasensitive color silver stain technique. Incubation of fat cells with insulin caused a 90% decrease in the plasma membrane concentration of a major plasma membrane protein with a molecular mass of 90 kDa. The insulin effect was dose-dependent with a half-maximal effect at 9.5 microunits/ml, and time-dependent with a t 1/2 of less than 20 s. Insulin-like growth factor I, orthovanadate, and lanthanum mimicked the effect of insulin. Likewise, fractionation of adipocytes in the presence of divalent cation chelating agents caused a similar reduction in the concentration of the 90 kDa protein, and it was possible to overcome the effects of the chelating agents by adding equivalent amounts of calcium. This suggests the involvement of calcium. The 90 kDa protein was also found in low and high density microsomes, but it was not affected in those fractions by either insulin or chelators. It is suggested from the study that the movement of a 90 kDa protein in fat cell plasma membranes probably represents part of the transmission system in the mechanism of insulin action in rat adipocytes.

Published

1984

91. Rapid method for homogenizing tissue samples for liquid scintillation counting.

Author

Adams LD, Curry LL, and Bartek MJ

Subjects

Freezing, Methods, Radiometry, Solubility, Time Factors, Chemistry Techniques, Analytical instrumentation, Connective Tissue analysis

Published

1970

92. Patient conformity in a Federal hospital for narcotic addicts.

Author

Adams LD, Michel JB, and Bates WM

Subjects

Acculturation, Drug and Narcotic Control, Humans, Length of Stay, Texas, United States, United States Public Health Service, Hospitals, Special, Prisons, Social Conformity, Substance-Related Disorders

Published

1970