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2. Detection of cytomegalovirus in the meconium of infected newborns by polymerase chain reaction

Author

Villanueva, M E, Svinarich, D M, Gonik, B, and Ostrea, E M

Subjects
Electrophoresis, Agar Gel, Meconium, Pregnancy, Cytomegalovirus Infections, DNA, Viral, Infant, Newborn, virus diseases, Cytomegalovirus, Humans, Female, Polymerase Chain Reaction, Sensitivity and Specificity, Research Article
Abstract

OBJECTIVE: Congenital cytomegalovirus (CMV) infection is a leading cause of hearing loss and mental retardation throughout the world. Detection of the CMV DNA by polymerase chain reaction (PCR) offers a sensitive, rapid, and specific means of identification. Meconium, the stool formed in utero, may be an ideal specimen for CMV detection. The objective of this study was to develop a PCR-based methodology for the detection of CMV in the meconium of neonates. METHODS: Meconium was collected from 10 newborn infants (seven with positive viral cultures and three uninfected infants born to CMV-seropositive mothers). For each, DNA was isolated from meconium by organic extraction and attachment to a DNA-binding matrix, and PCR was performed using amplimers specific for the major intermediate early (MIE) and late antigenic (LA) regions of CMV. RESULTS: Gel electrophoresis demonstrated an anticipated PCR product of 250 base pairs (bp) corresponding to the MIE region of CMV in all infected and positive control meconium samples. Furthermore, a single band of 150 bp corresponding to the LA region of CMV was also amplified in several of the infected infants. Conversely, no amplification of these antigenic regions was noted in either uninfected infants born to CMV-seropositive mothers or negative controls. CONCLUSIONS: CMV is present within the meconium of infected neonates and is readily detectable by PCR.

Published
2000

7. Ethanol-induced expression of cytokines in a first-trimester trophoblast cell line.

Author

Svinarich, David M., DiCerbo, John A., Zaher, Fadi M., Yelian, Frank D., Gonik, Bernard, Svinarich, D M, DiCerbo, J A, Zaher, F M, Yelian, F D, and Gonik, B

Subjects
FETAL immunology, CYTOKINES, ALCOHOL, BLASTOCYST, CELL lines, ETHANOL, GRANULOCYTE-colony stimulating factor, INTERLEUKINS, FIRST trimester of pregnancy, LIPOPOLYSACCHARIDES
Abstract

Objectives: Altered cytokine expression at the fetoplacental interface may be a potential mechanism for the development of fetal immune dysfunction in children with fetal alcohol syndrome. This study was conducted to determine whether first-trimester trophoblasts respond to ethanol exposure by the induction of specific cytokines.Study Design: HTR-8/SVneo trophoblast cells were cultured in vitro in the presence of either ethanol (0.5% [vol/vol]), lipopolysaccharide (1 microg/mL), or ethanol and lipopolysaccharide. Expression of granulocyte colony-stimulating factor, regulated on activation normal T cell expressed and secreted, and interleukin-6 was examined by Northern analysis and enzyme-linked immunosorbent assay.Results: Culture in the presence of ethanol, lipopolysaccharide, or lipopolysaccharide and ethanol resulted in the increased transcription and secretion of granulocyte colony-stimulating factor, regulated on activation normal T cell expressed and secreted, and interleukin-6 at significantly greater levels (P < .01) than control cultures.Conclusions: Human first-trimester trophoblasts express high levels of cytokines when cultured in the presence of ethanol. Trophoblasts may therefore be an important exogenous source of cytokines for the fetus, and altered cytokine levels during early gestation may have an adverse effect on the development of the fetal immune system. [ABSTRACT FROM AUTHOR]

Published
1998
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8. Association of adhesive, invasive, and virulent phenotypes of Salmonella typhimurium with autonomous 60-megadalton plasmids

Author

Jones, G W, Rabert, D K, Svinarich, D M, and Whitfield, H J

Abstract

The plasmid DNA content of six invasive and adhesive strains of Salmonella typhimurium was determined, and all six strains (CR8500 [S850], CR6600 [TML], W118, NY, PR, and S2204) were found to harbor at least one plasmid equivalent in size to the 60-megadalton plasmid ("cryptic" plasmid), pSLT, which is normally resident in S. typhimurium strain LT2. The role of such 60-megadalton plasmids in the adhesive and invasive properties of strain CR6600, a commonly encountered salmonella pathogen that produces type 1 fimbriae, and strain CR8500, a representative FIRN biotype which does not produce type 1 fimbriae, was studied further by obtaining derivatives of these strains that no longer harbored an autonomous 60-megadalton plasmid. Strains CR6260 and CR6190 and strains CR8100 and CR8353, which were "cured" derivatives of strains CR6600 and CR8500, respectively, were significantly less adhesive and invasive in the HeLa cell test. A 53.5-megadalton colicin plasmid harbored by strain CR6600 did not detectably influence these properties. Additionally, strain CR6260 was avirulent, and strain CR8100 was 1,000 to 10,000-fold less virulent for orally infected mice as compared with their respective parental strains. Significantly, the virulence of strain CR8100 correlated with tissue colonization by bacteria that exhibited autonomous copies of a 60-megadalton plasmid. We propose that this plasmid exists in both autonomous and integrated states and that the in vivo environment selects for bacteria with autonomous plasmid copies which can express the virulent phenotype, thus enabling such strains to survive the defense mechanisms of the host.

Published
1982
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9. Human primitive mesenchymal stem cell-derived retinal progenitor cells improved neuroprotection, neurogenesis, and vision in rd12 mouse model of retinitis pigmentosa.

Author

Brown C, Agosta P, McKee C, Walker K, Mazzella M, Alamri A, Svinarich D, and Chaudhry GR

Subjects
Animals, Disease Models, Animal, Humans, Mice, Neurogenesis, Neuroprotection, Retina metabolism, Stem Cells pathology, Mesenchymal Stem Cells pathology, Retinal Degeneration pathology, Retinitis Pigmentosa genetics, Retinitis Pigmentosa metabolism, Retinitis Pigmentosa therapy
Abstract

Background: Currently, there is no treatment for retinal degenerative diseases (RDD) such as retinitis pigmentosa (RP). Stem cell-based therapies could provide promising opportunities to repair the damaged retina and restore vision. Thus far, primarily adult mesenchymal stem cells (MSCs) have been investigated in preclinical and clinical studies, and the results have not been convincing. We applied a new approach in which primitive (p) MSC-derived retinal progenitor cells (RPCs) were examined to treat retinal degeneration in an rd12 mouse model of RP., Methods: Well-characterized pMSCs and RPCs labeled with PKH26 were intravitreally injected into rd12 mice. The vision and retinal function of transplanted animals were analyzed using electroretinography. Animals were killed 4 and 8 weeks after cell transplantation for histological, immunological, molecular, and transcriptomic analyses of the retina., Results: Transplanted RPCs significantly improved vision and retinal thickness as well as function in rd12 mice. pMSCs and RPCs homed to distinct retinal layers. pMSCs homed to the retinal pigment epithelium, and RPCs migrated to the neural layers of the retina, where they improved the thickness of the respective layers and expressed cell-specific markers. RPCs induced anti-inflammatory and neuroprotective responses as well as upregulated the expression of genes involved in neurogenesis. The transcriptomic analysis showed that RPCs promoted neurogenesis and functional recovery of the retina through inhibition of BMP and activation of JAK/STAT and MAPK signaling pathways., Conclusions: Our study demonstrated that RPCs countered inflammation, provided retinal protection, and promoted neurogenesis resulting in improved retinal structure and physiological function in rd12 mice., (© 2022. The Author(s).)

Published
2022
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10. Integration of Advance Care Planning Into Clinical Practice: A Quality Improvement Project for Leaders.

Author

Simmons-Fields L, Burgermeister D, Svinarich D, and Hanson P

Subjects
Evidence-Based Nursing, Humans, Professional Competence, Prospective Studies, Advance Care Planning organization & administration, Advance Care Planning statistics & numerical data, Delivery of Health Care, Integrated, Leadership, Nurse Administrators education, Quality Improvement
Abstract

Objective: This quality improvement initiative sought to develop a proactive integrated system approach to advance care planning (ACP) through leadership and colleague engagement., Background: Nurse leaders have the capacity to influence the professional competencies of care teams in ACP. Nurse leaders were educated on the importance of ACP, national quality metrics, resources for staff education, and ways to integrate ACP into workflows based on a population management model., Methods: The project design is a prospective, mixed method design., Results: Nurse leader participants demonstrated a significant increase in knowledge of the importance of ACP and evidence-based models to increase staff engagement and competency., Conclusions: Study supports nurse leader interventions, promoted engagement of proactive ACP to honor patient choice, and aligns with the mission and vision of one of the largest national Catholic healthcare organizations of being a trusted partner for life.

Published
2020
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11. Mesenchymal stem cells: Cell therapy and regeneration potential.

Author

Brown C, McKee C, Bakshi S, Walker K, Hakman E, Halassy S, Svinarich D, Dodds R, Govind CK, and Chaudhry GR

Subjects
Clinical Trials as Topic, Fetus cytology, Humans, Mesenchymal Stem Cell Transplantation, Mesenchymal Stem Cells cytology, Regeneration
Abstract

Rapid advances in the isolation of multipotent progenitor cells, routinely called mesenchymal stromal/stem cells (MSCs), from various human tissues and organs have provided impetus to the field of cell therapy and regenerative medicine. The most widely studied sources of MSCs include bone marrow, adipose, muscle, peripheral blood, umbilical cord, placenta, fetal tissue, and amniotic fluid. According to the standard definition of MSCs, these clonal cells adhere to plastic, express cluster of differentiation (CD) markers such as CD73, CD90, and CD105 markers, and can differentiate into adipogenic, chondrogenic, and osteogenic lineages in vitro. However, isolated MSCs have been reported to vary in their potency and self-renewal potential. As a result, the MSCs used for clinical applications often lead to variable or even conflicting results. The lack of uniform characterization methods both in vitro and in vivo also contributes to this confusion. Therefore, the name "MSCs" itself has been increasingly questioned lately. As the use of MSCs is expanding rapidly, there is an increasing need to understand the potential sources and specific potencies of MSCs. This review discusses and compares the characteristics of MSCs and suggests that the variations in their distinctive features are dependent on the source and method of isolation as well as epigenetic changes during maintenance and growth. We also discuss the potential opportunities and challenges of MSC research with the hope to stimulate their use for therapeutic and regenerative medicine., (© 2019 John Wiley & Sons, Ltd.)

Published
2019
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13. In vivo intervertebral disc regeneration using stem cell-derived chondroprogenitors.

Author

Sheikh H, Zakharian K, De La Torre RP, Facek C, Vasquez A, Chaudhry GR, Svinarich D, and Perez-Cruet MJ

Subjects
Animals, Disease Models, Animal, Female, Rabbits, Regeneration physiology, Chondrocytes cytology, Embryonic Stem Cells transplantation, Guided Tissue Regeneration methods, Intervertebral Disc physiology, Lumbar Vertebrae, Spondylosis therapy
Abstract

Object: There is currently no biologic therapy to repair or restore a degenerated intervertebral disc. A potential solution may rest with embryonic stem cells (ESCs), which have a potential to grow indefinitely and differentiate into a variety of cell types in vitro. Prior studies have shown that ESCs can be encouraged to differentiate toward specific cell lineages by culture in selective media and specific growth environment. Among these lineages, there are cells capable of potentially producing nucleus pulposus (NP) in vivo. In this investigation, the authors studied ESCderived chondroprogenitors implanted into a degenerated disc in a rabbit. For this purpose, a rabbit model of disc degeneration was developed., Methods: A percutaneous animal model of disc degeneration was developed by needle puncture of healthy intact discs in 16 New Zealand white rabbits. Series of spine MR imaging studies were obtained before disc puncture and after 2, 6, and 8 weeks. Prior to implantation, murine ESCs were cultured with cis-retinoic acid, transforming growth factor beta, ascorbic acid, and insulin-like growth factor to induce differentiation toward a chondrocyte lineage. After confirmation by MR imaging, degenerated disc levels were injected with chondrogenic derivatives of ESCs expressing green fluorescent protein. At 8 weeks post-ESC implantation, the animals were killed and the intervertebral discs were harvested and analyzed using H & E staining, confocal fluorescent microscopy, and immunohistochemical analysis. Three intervertebral disc groups were analyzed in 16 rabbits, as follows: 1) Group A, control: naïve, nonpunctured discs (32 discs, levels L4-5 and L5-6); 2) Group B, experimental control: punctured disc (16 discs, level L2-3); and 3) Group C, experimental: punctured disc followed by implantation of chondroprogenitor cells (16 discs, level L3-4)., Results: The MR imaging studies confirmed intervertebral disc degeneration at needle-punctured segments starting at approximately 2 weeks. Postmortem H & E histological analysis of Group A discs showed mature chondrocytes and no notochordal cells. Group B discs displayed an intact anulus fibrosus and generalized disorganization within fibrous tissue of NP. Group C discs showed islands of notochordal cell growth. Immunofluorescent staining for notochordal cells was negative for Groups A and B but revealed viable notochordal-type cells within experimental Group C discs, which had been implanted with ESC derivatives. Notably, no inflammatory response was noted in Group C discs., Conclusions: This study illustrates a reproducible percutaneous model for studying disc degeneration. New notochordal cell populations were seen in degenerated discs injected with ESCs. The lack of immune response to a xenograft of mouse cells in an immunocompetent rabbit model may suggest an as yet unrecognized immunoprivileged site within the intervertebral disc space.

Published
2009
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14. Adhesion development and the expression of endothelial nitric oxide synthase.

Author

Svinarich DM, Zaher FM, Holmdahl L, Chegini N, Gonik B, and Diamond MP

Subjects
Actins analysis, Endothelium physiopathology, Female, Gene Expression Profiling, Humans, Peritoneal Diseases genetics, Peritoneum physiopathology, Pilot Projects, Reverse Transcriptase Polymerase Chain Reaction, Skin physiopathology, Tissue Adhesions genetics, Nitric Oxide Synthase physiology, Peritoneal Diseases physiopathology, RNA, Messenger analysis, Tissue Adhesions physiopathology
Abstract

Objective: This study was conducted to determine whether nitric oxide (NO), a potent vasodilator and inhibitor of thrombus formation, is involved in the formation and maintenance of adhesions., Methods: Skin, subcutaneous tissues, peritoneum and adhesions were collected from surgical patients and total RNA was isolated. Quantitative reverse transcription polymerase chain reaction (QRT-PCR) was performed to quantitate endothelial nitric oxide synthase (eNOS) and beta-actin mRNA levels., Results: eNOS mRNA levels for skin, subcutaneous tissue, peritoneum and adhesions were < or = 3.12 x 10(-4), < or = 3.12 x 10(-4), 6.24 x 10(-4) and 2.5 x 10(-3) attomoles/microl, respectively. Beta-actin mRNA levels for all tissues were between 1.25 x 10(-1) and 6.25 x 10(-2) attomoles/microl., Conclusion: eNOS mRNA can be identified in tissue adhesions, and may therefore play a role in adhesion formation and maintenance.

Published
2001
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15. Expression and regulation of vascular endothelial growth factor in a first trimester trophoblast cell line.

Author

Chung IB, Yelian FD, Zaher FM, Gonik B, Evans MI, Diamond MP, and Svinarich DM

Subjects
Adult, Blotting, Northern, Cell Line, Transformed, Enzyme-Linked Immunosorbent Assay, Female, Gene Expression Regulation, Humans, Oligonucleotide Probes chemistry, Pregnancy, Pregnancy Trimester, First, RNA analysis, Transforming Growth Factor beta pharmacology, Trophoblasts cytology, Trophoblasts drug effects, Tumor Necrosis Factor-alpha pharmacology, Vascular Endothelial Growth Factor A, Vascular Endothelial Growth Factors, Endothelial Growth Factors genetics, Lymphokines genetics, RNA, Messenger biosynthesis, Trophoblasts metabolism
Abstract

Embryo implantation and development are critically dependent upon the spatial and temporal regulation of angiogenesis and localized vascular permeability. A key mediator of these effects is the endothelial cell mitogen vascular endothelial growth factor (VEGF). VEGF has been shown to promote endometrial vascular permeability, fetal vasculogenesis and placental, fetal and maternal angiogenesis. However, the mechanism through which this regulation occurs in the placenta is poorly understood. This study was conducted to determine if the pro-angiogenic cytokines, TNF-alpha and TGF-beta1, affect VEGF expression in human first trimester trophoblasts. Culture of a first trimester trophoblast cell line (HTR-8/SVneo), in the presence of either TNF-alpha or TGF-beta1, resulted in the expression of significant levels of VEGF in culture. The trophoblast cell line also showed a time-dependent and a dose-dependent increase in VEGF mRNA levels when cultured in the presence of either TNF-alpha or TGF-beta1. These results suggest that both TNF-alpha and TGF-beta1 may regulate the production of VEGF in early gestational trophoblasts and may therefore serve to modulate placental vascular permeability and angiogenesis that are necessary for embryo implantation and placentation., (Copyright 2000 Harcourt Publishers Ltd.)

Published
2000
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16. Effect of imiquimod on cytokine induction in first trimester trophoblasts.

Author

Manlove-Simmons JM, Zaher FM, Tomai M, Gonik B, and Svinarich DM

Subjects
Cell Line, Cell Survival drug effects, Cell Survival physiology, Dose-Response Relationship, Drug, Female, Humans, Imiquimod, Pregnancy, Pregnancy Trimester, First, Reverse Transcriptase Polymerase Chain Reaction, Sensitivity and Specificity, Trophoblasts cytology, Aminoquinolines pharmacology, Cytokines biosynthesis, Cytokines drug effects, Interferon Inducers pharmacology, RNA analysis, Trophoblasts metabolism
Abstract

Objectives: Imiquimod (IQ) is used clinically for the topical treatment of external genital warts. IQ is an immune response modifier and induces the expression of interferon-alpha and other cytokines in human Peripheral Blood Monocytes (PBMC). Trophoblasts have been previously shown to express inflammatory cytokines upon lipopolysaccharide (LPS) stimulation. The objective of this study was to evaluate the ability of IQ to induce transcription of cytokines in trophoblasts., Methods: A transformed human first trimester trophoblast cell line, HTR-8/SVneo, was cultured in DMEM containing IQ at concentrations of 0 to 5.0 microg/ml. 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide (MTT) viability assays were conducted to control for any drug-induced cell death. Total RNA was isolated from trophoblasts at 0, 8 and 24 hours of culture and Reverse Transcription-Polymerase Chain Reaction (RT-PCR) was conducted using specific amplimers for the inflammatory cytokines interleukin (IL)-1alpha, IL-1beta, IL-6 and IL-8. RT-PCR of beta-actin was performed to control for equal RNA loading., Results: RT-PCR was unable detect an increase in either IL-1alpha, IL-1beta, IL-6 or IL-8 mRNA in first trimester trophoblasts cultured in the presence of 0 to 5.0 microg/mL of IQ for up to 24 hours. RT-PCR confirmed equal RNA loading and MTT viability assays did not show loss of cell viability at concentrations of IQ up to 5.0 microg/ml., Conclusions: IQ, at the concentrations tested, did not induce the transcriptional expression of inflammatory cytokines in human first trimester trophoblasts. These data suggest that IQ would not induce the expression of inflammatory cytokines in placental trophoblasts.

Published
2000
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17. Decreased gene expression of endothelial nitric oxide synthase in newborns with persistent pulmonary hypertension.

Author

Villanueva ME, Zaher FM, Svinarich DM, and Konduri GG

Subjects
Cells, Cultured, Endothelium, Vascular pathology, Humans, Infant, Newborn, Nitric Oxide Synthase biosynthesis, Nitric Oxide Synthase Type III, Persistent Fetal Circulation Syndrome enzymology, Persistent Fetal Circulation Syndrome pathology, Polymerase Chain Reaction, Umbilical Cord, Endothelium, Vascular enzymology, Gene Expression Regulation, Enzymologic, Nitric Oxide Synthase genetics, Persistent Fetal Circulation Syndrome genetics
Abstract

Previous studies in adults have shown that chronic pulmonary hypertension is associated with decreased endothelial nitric oxide synthase (eNOS) expression in pulmonary arteries. However, the role of decreased eNOS expression in persistent pulmonary hypertension of the newborn (PPHN) is unknown. We investigated the hypothesis that umbilical vein endothelial cells cultured from infants with PPHN will have decreased eNOS expression. Umbilical cords were collected from meconium-stained infants at birth, and endothelial cells were isolated if the infants developed PPHN. Endothelial cells were grown in primary culture, and total RNA was isolated. cDNA was reverse transcribed from mRNA and amplified by PCR. An expected product of approximately 550 bp was found in all control infants but only in two of the six infants with PPHN. Identity of the PCR product was confirmed by Southern hybridization to a separate internal eNOS-specific probe. Amplification of beta-actin cDNA, an internal control, was detected in all controls and in all infants with PPHN, including the four infants without the eNOS band. There was no difference in the course and outcome of patients with presence or absence of the eNOS band. However, there was an acidotic arterial blood pH (7.19-7.29) and intrapartum fetal heart rate decelerations in all four infants without eNOS expression. In conclusion, eNOS mRNA was detected in all normal term infants but was notably absent in the majority of infants with PPHN in this pilot study. The development of PPHN is multifactorial, and a decrease in eNOS gene expression may occur in some infants. Whether the decreased eNOS transcript is a cause of PPHN or a result of intrapartum stress remains to be determined.

Published
1998
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18. Detection of human defensins in the placenta.

Author

Svinarich DM, Gomez R, and Romero R

Subjects
Amnion immunology, Amnion metabolism, Base Sequence, Blood Proteins genetics, Blood Proteins immunology, Chorion immunology, Chorion metabolism, DNA Primers genetics, DNA, Complementary genetics, Defensins, Female, Gene Expression, Humans, Molecular Sequence Data, Pregnancy, Pregnancy Complications, Infectious immunology, Pregnancy Complications, Infectious prevention & control, Random Amplified Polymorphic DNA Technique, Blood Proteins metabolism, Placenta immunology, Placenta metabolism
Abstract

Problem: The placenta is a highly selective barrier against the hematogenous dissemination of infectious agents. Despite the presence of seemingly intact physical and immunologic barriers, infections nonetheless occur. These observations prompted the examination of placental tissue, amnion, and chorion for previously unrecognized protective mechanisms., Method of Study: Messenger RNA from term placenta, amnion, and chorion were reverse transcribed using a 3' RACE adapter. 3' rapid amplification of cDNA ends (RACE)-polymerase chain reaction (PCR) was conducted on cDNA from these tissues to detect the presence of human defensins. Southern analysis and partial sequence analysis were subsequently performed to confirm identity., Results: PCR amplification of placental, amnion, and chorion cDNA yielded a 468-bp product and a weakly detectable band of 300 bp. Southern analysis demonstrated two corresponding hybridizing bands in the placenta, amnion, and chorion but not from a negative cDNA control. Partial sequence analysis of the 468-bp product from placenta confirmed the presence of either defensin 1 or 3 in human placenta., Conclusions: The human placenta, amnion, and chorion express defensins at the level of transcription. These findings suggest that a novel and previously unrecognized mechanism of protecting the fetus against infection may be present within these tissues.

Published
1997
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19. Detection of human defensin 5 in reproductive tissues.

Author

Svinarich DM, Wolf NA, Gomez R, Gonik B, and Romero R

Subjects
Amnion chemistry, Base Sequence, Biomarkers analysis, Cell Line, Cervix Uteri chemistry, Chorion chemistry, Defensins, Endometrium chemistry, Female, Humans, Intestine, Small chemistry, Lymphocytes chemistry, Molecular Sequence Data, Myometrium chemistry, Placenta chemistry, Polymerase Chain Reaction methods, Blood Proteins analysis, Extraembryonic Membranes chemistry, Genitalia, Female chemistry
Abstract

Objectives: This study was undertaken to determine whether tissue-specific defensins are expressed within female reproductive tissues., Study Design: Messenger ribonucleic acid from amnion, chorion, endometrium, endocervix, myometrium, placenta, small intestine, peripheral blood lymphocytes, and cervical, endometrial, and trophoblast cell lines was reverse transcribed with a 3'-RACE adapter. 3'-RACE polymerase chain reaction was conducted with an upstream human defensin 5 primer and 3'-RACE adapter primer. Polymerase chain reaction products hybridizing to a human defensin 5 probe were cloned for sequence analysis. Sequence data were compared against a nucleotide sequence database, and secondary structure predictions were made., Results: Chorionic tissue, endocervical tissue, endometrial tissue, and an endometrial cell line all demonstrated a single hybridizing 362 bp polymerase chain reaction product. Sequence analysis of all clones demonstrated near-perfect identity with human defensin 5., Conclusions: Human endocervix, endometrium, and chorion express defensin 5 at the level of transcription. These findings suggest that a previously unrecognized mechanism of protecting female reproductive tissues against infection, by means of a natural antimicrobial system (defensins), may be present.

Published
1997
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20. Induction and postranslational expression of G-CSF and RANTES in a first trimester trophoblast cell line by lipopolysaccharide.

Author

Svinarich DM, Bitonti OM, Araneda H, Romero R, and Gonik B

Subjects
Blotting, Northern, Cell Line metabolism, Enzyme-Linked Immunosorbent Assay, Female, Humans, Nucleic Acid Hybridization, Pregnancy, Pregnancy Trimester, First, RNA, Chemokine CCL5 metabolism, Granulocyte Colony-Stimulating Factor metabolism, Lipopolysaccharides pharmacology, Protein Processing, Post-Translational drug effects, Trophoblasts cytology
Abstract

Problem: Comparatively little is known about the capacity of first trimester trophoblasts to respond to an infection and coordinate an immune response. This study characterizes the LPS induction of G-CSF and RANTES in a first trimester trophoblast cell line., Methods: HTR-8/SV neo cells were exposed to LPS (1 micrograms/ml) for 0, 2, 4, 6, 8, and 24 hours in DMEM-Ham's F-12 media supplemented with 10% fetal bovine serum. Cytokine levels in culture supernatants were measured by ELISA. Northern analysis of total RNA was conducted using antisense cytokine probes., Results: Levels of immunoreactive G-CSF and RANTES from LPS induced cultures at 24 hours were 10-fold and 8.5-fold greater than cytokine levels from non-induced cells at 24 hours, respectively (P < 0.01). Under LPS induction, maximal rates of G-CSF and RANTES transcription occurred at 24 hours and 8 hours, respectively., Conclusion: The LPS induction of proinflammatory cytokines in a first trimester trophoblast cell line supports the contention that first trimester trophoblasts participate in cytokine based immune signaling in response to infection.

Published
1996
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21. Induction and posttranslational expression of cytokines in a first-trimester trophoblast cell line by lipopolysaccharide.

Author

Svinarich DM, Bitonti OM, Romero R, and Gonik B

Subjects
Blotting, Northern, Cell Line, Enzyme-Linked Immunosorbent Assay, Female, Humans, Interleukins genetics, Interleukins metabolism, Pregnancy, RNA, Messenger metabolism, Time Factors, Transforming Growth Factor beta genetics, Transforming Growth Factor beta metabolism, Cytokines metabolism, Lipopolysaccharides pharmacology, Pregnancy Trimester, First, Protein Processing, Post-Translational, Trophoblasts drug effects, Trophoblasts metabolism
Abstract

Objectives: The response to infection by human first-trimester trophoblasts is a poorly understood event. This study was undertaken to determine whether first-trimester trophoblasts are capable of responding to an infection stimulus and mediating an immune response., Study Design: HTR-8/SVneo cells were exposed to lipopolysaccharide (1 microgram/ml) or media alone for either 0, 2, 4, 6, 8, or 24 hours. Northern analysis was conducted by use of a panel of antisense cytokine probes. Enzyme-linked immunosorbent assays specific for either interleukin-1 alpha, interleukin-6, interleukin-8, or transforming growth factor-beta 1 were conducted on corresponding cell culture supernatants, and the kinetics of expression were determined., Results: Interleukin-1 alpha, interleukin-6, interleukin-8, and transforming growth factor-beta 1 transcription occurred maximally between 2 and 8 hours of culture in media containing lipopolysaccharide, with a subsequent diminution of response. Enzyme-linked immunosorbent assay analysis corroborated lipopolysaccharide induction seen at the level of transcription, with significant posttranslational expression of these cytokines being detected between 2 and 24 hours in culture (p < 0.01)., Conclusions: Expression of the proinflammatory cytokines interleukin-1 alpha, interleukin-6, interleukin-8 and transforming growth factor-beta 1 strongly support the contention that human first-trimester trophoblasts are capable of responding to an infection stimulus and eliciting an immune response through cytokine-based immune signaling.

Published
1996
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22. Human trophoblast cell adhesion to extracellular matrix protein, entactin.

Author

Yang Y, Todt JC, Svinarich DM, Qureshi F, Jacques SM, Graham CH, Chung AE, Gonik B, and Yelian FD

Subjects
Antigens, CD biosynthesis, Basement Membrane metabolism, Cell Adhesion, Cell Line, Flow Cytometry, Fluorescent Antibody Technique, Indirect, Humans, Integrin beta3, Integrins biosynthesis, Placenta cytology, Platelet Membrane Glycoproteins biosynthesis, Protein Binding immunology, Protein Conformation, Receptors, Vitronectin biosynthesis, Trophoblasts cytology, Extracellular Matrix Proteins metabolism, Membrane Glycoproteins metabolism, Trophoblasts metabolism
Abstract

Problem: Trophoblast interaction with endometrial extracellular matrix (ECM) is crucial during human embryo implantation and placentation. Entactin, a ubiquitous basement membrane glycoprotein, plays a central role in ECM assembly, cell attachment, and chemotaxis. The present study was conducted to examine the possible role of entactin in promoting human trophoblast adhesion., Methods: Using an extended life span first trimester trophoblast cell line HTR-8/SVneo (HTR) and a cell adhesion assay, we measured the adherence of human first trimester trophoblasts to recombinant entactin and its domains. Also, we used flow cytometry and indirect immunofluorescence to detect the presence of integrins that may be involved in human trophoblast-entactin interaction; these methods were used to analyze HTR cells, as well as tissue sections and freshly isolated human trophoblasts from first trimester and term placenta., Results: We found that first trimester trophoblast cells were highly adherent to entactin and its E and G2 domains but not to G1 or G3 domains. Using indirect immunofluorescence and flow cytometry, we found that both beta 1 and beta 3 integrin subunits were expressed on the surface of HTR trophoblast cells adhering to entactin; in contrast, beta 2 and beta 4 integrin subunits were not detected. In addition, we found that alpha v beta 3 was expressed on freshly isolated villous cytotrophoblasts and cytotrophoblast and syncytiotrophoblasts in tissue sections from term placenta. The beta 3 integrin subunit was expressed in cytotrophoblasts and syncytiotrophoblasts in villi of first trimester placental tissue sections., Conclusion: Recombinant entactin promotes human trophoblast cell adhesion through both its E and G2 domains and these specific adhesive interactions may be mediated by beta 1 and/or beta 3 class integrins.

Published
1996
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23. Macrophage inflammatory protein-1 alpha in term and preterm parturition: effect of microbial invasion of the amniotic cavity.

Author

Romero R, Gomez R, Galasso M, Munoz H, Acosta L, Yoon BH, Svinarich D, and Cotton DB

Subjects
Amniotic Fluid immunology, Amniotic Fluid microbiology, Chemokine CCL4, Female, Gestational Age, Humans, Macrophage Inflammatory Proteins, Pregnancy, Amnion immunology, Amnion microbiology, Cytokines analysis, Labor, Obstetric immunology, Monokines analysis, Obstetric Labor, Premature immunology
Abstract

Problem: This study was conducted to determine whether: (1) gestational age, parturition, and microbial invasion of the amniotic cavity (MIAC) are associated with changes in amniotic fluid concentrations of immunoreactive macrophage inflammatory protein-1 alpha; (2) amniotic fluid concentrations of macrophage inflammatory protein-1 alpha are correlated with the white blood cell count and the concentrations of interleukin-8 in amniotic fluid., Method: Amniotic fluid was retrieved by amniocentesis from 126 patients; 54 women with preterm labor and intact membranes (no MIAC-delivery at term, N = 21; no MIAC-preterm delivery, N = 16; MIAC-preterm delivery, N = 17); 62 patients at term (no labor, N = 19; labor-no MIAC, N = 20; labor-MIAC, N = 23); and 10 patients in the midtrimester of pregnancy. Amniotic fluid was cultured for aerobic, anaerobic and Mycoplasma species. Determinations of amniotic fluid macrophage inflammatory protein-1 alpha and interleukin-8 were performed with immunoassays validated for amniotic fluid (sensitivity: 14.2 pg/ml and 0.3 ng/ml, respectively). Kruskal-Wallis analysis of variance (ANOVA) for censored data, Mann-Whitney U test and Spearman's rank correlation were performed for analysis., Results: 1) Amniotic fluid macrophage inflammatory protein-1 alpha was present in only 31.0% (9/29) of patients not in labor (midtrimester and term). 2) Patients with preterm labor and MIAC had higher amniotic fluid concentrations of macrophage inflammatory protein-1 alpha than those without MIAC (no MIAC-delivery at term: median 0.0 pg/ml, range 0.0-221.2; no MIAC-preterm delivery: median 37.4 pg/ml, range 0.0-494.6; MIAC-preterm delivery: median 7171.0 pg/ml, range 402.5-37994.0; P < 0.00001). 3) Among patients at term, MIAC was associated with higher concentrations of amniotic fluid macrophage inflammatory protein-1 alpha than patients without MIAC (no labor: median 0.0 pg/ml, range 0.0-25.6; labor-no MIAC: median 16.7 pg/ml, range 0.0-161.6; labor-MIAC: median 103.8 pg/ml, range 0.0-4349.0, P < 0.001). 4) Among patients in preterm labor, a strong correlation was found between amniotic fluid concentrations of macrophage inflammatory protein-1 alpha and interleukin-8 (r = 0.9, P < 0.00001) and between amniotic fluid macrophage inflammatory protein-1 alpha concentrations and amniotic fluid white blood cell count (r = 0.6, P < 0.0001)., Conclusions: (1) Macrophage inflammatory protein-1 alpha is undetectable in most amniotic fluid samples from patients in the midtrimester of pregnancy and at term not in labor. (2) Microbial invasion of the amniotic cavity is associated with increased concentrations of immunoreactive amniotic fluid macrophage inflammatory protein-1 alpha in both term and preterm gestations. (3) Amniotic fluid macrophage inflammatory protein-1 alpha concentrations significantly correlate with interleukin-8 levels and white blood cell count in amniotic fluid. Our data strongly suggest a role for macrophage inflammatory protein-1 alpha in the mechanisms responsible for the recruitment of leukocytes into the amniotic cavity during the course of intrauterine infection.

Published
1994
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24. The mouse lysyl oxidase gene (Lox) resides on chromosome 18.

Author

Chang YS, Svinarich DM, Yang TP, and Krawetz SA

Subjects
Animals, Blotting, Southern, Cricetinae, Hybrid Cells, Mice genetics, Protein-Lysine 6-Oxidase genetics
Abstract

Lysyl oxidase initiates crosslink formation of the connective tissue matrix. This enzyme can also revert the ras phenotype in mouse NIH 3T3-transformed cells. Even though lysyl oxidase may participate in many different biological processes, its chromosomal assignment in the mouse genome remains to be addressed. Southern analysis of a panel of Chinese hamster x mouse somatic cell hybrids was utilized to assign the lysyl oxidase gene (Lox) to mouse Chromosome 18.

Published
1993
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25. Gene assignment by quantitative hybridization analysis of somatic cell hybrids.

Author

Svinarich DM and Krawetz SA

Subjects
Animals, Biotechnology, Evaluation Studies as Topic, Humans, Molecular Probes, Protein-Lysine 6-Oxidase genetics, Chromosome Mapping methods, Hybrid Cells ultrastructure, Nucleic Acid Hybridization methods
Abstract

Since the inception of somatic cell hybridization technology, the number of genes mapped to a particular chromosome or region of a chromosome has increased exponentially. Conventional assignment relies on the interpretation and designation of concordance to the various panel members. Assignment of genes to individual chromosomes may be ambiguous if the representation of the individual chromosomes within the hybrid panel is not considered. To overcome this inherent limitation, we have developed a computer-assisted method to assign genes to chromosomes. This assignment utilizes an integrative statistical analysis procedure to reconcile chromosomal representation of each member of the somatic cell hybrid panel. In this manner, the intensity of the corresponding bands appearing on the autoradiographic image reflects the prevalence of that specific gene-containing chromosome within the somatic cell hybrid. The statistical method described above provides the foundation for an independent means to assign genes to a specific chromosome. We have utilized this method to assign the human lysyl oxidase gene to chromosome 5.

Published
1993

26. Regulation of the SLT-1A toxin operon by a ferric uptake regulatory protein in toxinogenic strains of Shigella dysenteriae type 1.

Author

Svinarich DM and Palchaudhuri S

Subjects
Bacterial Toxins genetics, Cytotoxins genetics, Escherichia coli genetics, Humans, Iron metabolism, Shiga Toxin 1, Shiga Toxins, Bacterial Proteins genetics, Bacterial Toxins biosynthesis, Gene Expression Regulation, Bacterial, Operon, Repressor Proteins genetics, Shigella dysenteriae genetics
Abstract

The regulation of Shiga toxin expression in a clinical isolate of S. dysenteriae 1 by the Fe-Fur (Iron-ferric uptake regulatory protein) repressor complex was investigated. The presence of an endogenous Fur repressor protein capable of binding to either a Fur binding consensus sequence or the regulatory region of SLT-1A was determined in toxinogenic strains of S. dysenteriae. Plasmid constructs bearing Fur binding sites fused to readily assayable reporter genes were used. Plasmid pSC27.1 contains a 21 bp synthetic oligonucleotide Fur protein binding consensus sequence located upstream to the gene for beta-galactosidase. Plasmid pSC105 contains the regulatory sequences of Shiga-like toxin-1A located upstream to the gene for alkaline phosphatase. In an analogous fashion to Shiga toxin regulation in S. dysenteriae 1, transformants bearing either pSC27.1 or pSC105 plasmid DNA were repressed in gene product expression when grown in minimal medium supplemented with iron. Conversely, transformants were de-repressed when grown under iron limiting conditions. These data suggest the presence of Fe-Fur mediated regulation of toxinogenesis in clinical isolates of S. dysenteriae.

Published
1992

27. Characterization of the human lysyl oxidase gene locus.

Author

Svinarich DM, Twomey TA, Macauley SP, Krebs CJ, Yang TP, and Krawetz SA

Subjects
Adult, Animals, Base Sequence, Blotting, Northern, Cells, Cultured, DNA genetics, DNA isolation & purification, Fetus, Fibroblasts enzymology, Genes, Tumor Suppressor, Humans, Mice, Molecular Sequence Data, Oligodeoxyribonucleotides, RNA, Messenger genetics, Rats, Restriction Mapping, Sequence Homology, Nucleic Acid, Skin enzymology, Software, Transcription, Genetic, Chromosome Mapping, Genes, Protein-Lysine 6-Oxidase genetics
Abstract

Lysyl oxidase (EC 1.4.3.13) is a copper-dependent enzyme acting principally on collagen and elastin catalyzing the formation of aldehyde cross-links. It is also believed to possess a tumor suppressor activity as the anti-oncogene of ras. While rat, human, and mouse lysyl oxidase cDNAs have been cloned, little is known about the structure of the gene, its organization, or regulation. This paper describes the cloning of an intronic segment of the human lysyl oxidase gene. Sequence analysis defined the location of an intron that separates the prepro-coding segments from the segment encoding the catalytic domain. Genomic restriction mapping and gene copy number data established that multiple lysyl oxidase mRNA transcripts originate from a single gene and thus are products of alternative splicing. Northern analysis of adult and fetal fibroblast RNA showed a dominant approximately 4.3-kilobase lysyl oxidase mRNA transcript that varied in abundance as a function of cell line. These data are consistent with a complex mechanism regulating the expression of the lysyl oxidase gene.

Published
1992

28. The stability of O-antigen plasmid is determined by a chromosomal region of Shigella dysenteriae 1.

Author

Aqua MS, Svinarich D, Dhar A, and Palchaudhuri S

Subjects
Antigens, Bacterial analysis, Antigens, Bacterial biosynthesis, Escherichia coli genetics, Histidine, Lipopolysaccharides analysis, O Antigens, Oligosaccharides analysis, Recombination, Genetic, Shigella dysenteriae analysis, Shigella dysenteriae immunology, Antigens, Bacterial genetics, Genes, Bacterial, Plasmids, Shigella dysenteriae genetics
Abstract

It is well established that plasmids are involved in the expression of lipopolysaccharide in certain species of Shigella. In Shigella sonnei, both the biosynthesis of oligosaccharide side chains (O antigen), and cell invasiveness are controlled exclusively by a 120 megadalton (MDa) plasmid. In Shigella dysenteriae 1, a 10 kilobase (kb) plasmid is required for O-antigen production. Shigella dysenteriae 1 strains devoid of this plasmid lose the ability to synthesize O antigen. Interestingly, this 10-kb plasmid is not stably maintained in Escherichia coli K-12 strains, where it is lost spontaneously at a high frequency. Our genetic analyses of Shigella dysenteriae 1 strain IDBM11 and its derivatives indicate that the stability of this plasmid is associated with the histidine region of the chromosome which is unique to Shigella dysenteriae. Furthermore, the 10-kb plasmid is stably maintained in wild-type IDBM11 with an intact histidine locus. However, this plasmid is not stable in IDBM11 derivatives (e.g., IDBM11-1 and IDBM11-2), in which the his locus has been substituted with the histidine region of an E. coli K-12 chromosome. The S. dysenteriae IDBM11 strain, and its derivatives (lacking a 10-kb plasmid), displayed an invasive property as demonstrated by their internalization by HeLa cells in an in vitro assay. Thus the 10-kb plasmid of Shigella dysenteriae 1 is required for O-antigen synthesis but not for cell invasion.

Published
1988
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