Your search keyword '"Chatis P"' showing total 29 results

1. Simple Things You Can Do To Help All Children Read Well and Independently by the Third Grade. America Reads Challenge: Read*Write*Now!

Author

Department of Education, Washington, DC., Chatis, Corey, Thompson-Hoffman, Susan, de Kanter, Adriana, Moles, Ollie, Steele, Shirley, Howes, Sarah, Doyle, Michelle, Colmenares, Margarita, Vosburgh, Leah, Herman, Menahem, Ballen, Jennifer, and Arnold, Chandler

Abstract

This booklet presents suggestions for things people can do to help meet the America Reads Challenge of having all children read well and independently by the end of third grade. One of the ways to meet this challenge is through the research-based community reading initiative, called READ*WRITE*NOW!, which encourages students to read and write at least 30 minutes a day for 5 days a week. The introduction discusses how to start an after-school, weekend, or summer literacy program. The booklet then presents simple things that families, child care providers, schools, librarians, grandparents, seniors, and concerned citizens, community, cultural, and religious organizations, universities, employers, and the media can do to help. Contains a list of seven America Reads Challenge materials and addresses of 18 public and private organizations that are sources of literacy information. (RS)

Published

1997

2. Imatinib-induced regression of AIDS-related Kaposi's sarcoma.

Author

Koon HB, Bubley GJ, Pantanowitz L, Masiello D, Smith B, Crosby K, Proper J, Weeden W, Miller TE, Chatis P, Egorin MJ, Tahan SR, and Dezube BJ

Subjects

Administration, Oral, Antineoplastic Agents administration & dosage, Antineoplastic Agents adverse effects, Benzamides, Biopsy, Diarrhea chemically induced, Follow-Up Studies, Humans, Imatinib Mesylate, Male, Pilot Projects, Piperazines administration & dosage, Piperazines adverse effects, Protein Kinase Inhibitors administration & dosage, Protein Kinase Inhibitors adverse effects, Proto-Oncogene Proteins c-kit drug effects, Pyrimidines administration & dosage, Pyrimidines adverse effects, Receptors, Platelet-Derived Growth Factor antagonists & inhibitors, Remission Induction, Signal Transduction drug effects, Vascular Endothelial Growth Factor A blood, AIDS-Related Opportunistic Infections drug therapy, Antineoplastic Agents therapeutic use, Piperazines therapeutic use, Protein Kinase Inhibitors therapeutic use, Protein-Tyrosine Kinases antagonists & inhibitors, Pyrimidines therapeutic use, Sarcoma, Kaposi drug therapy, Skin Neoplasms drug therapy

Abstract

Purpose: Activation of the platelet-derived growth factor (PDGF) and c-kit receptors has been proposed as important in mediating the growth of AIDS-related Kaposi's sarcoma (KS). We investigated the response of KS to the PDGF receptor (PDGFR)/c-kit inhibitor, imatinib mesylate, and investigated the effect of this therapy on critical signal transduction intermediates., Patients and Methods: Ten male patients with AIDS-related cutaneous KS, which progressed despite chemotherapy and/or highly active antiretroviral therapy, received imatinib mesylate administered orally, 300 mg twice daily. Clinical response was determined by serial tumor measurements. To determine biologic and histologic response, skin lesion biopsies were obtained at baseline and following 4 weeks of therapy., Results: Five of 10 participants had a partial response by tumor measurements. Biopsies after 4 weeks of therapy demonstrated histologic regression in four of six patients. Four patients' tumor biopsies were assessable for immunohistochemistry end points pre- and post-therapy. These demonstrated inhibition of PDGFR and its downstream effector, extracellular receptor kinase, which is a member of the mitogen-activated protein kinase family. The most common adverse event was diarrhea, which led to dose reduction in six patients., Conclusion: Imatinib mesylate administered orally twice daily for AIDS-related KS results in clinical and histologic regression of cutaneous KS lesions within 4 weeks. These promising results demonstrate that inhibition of the c-kit and/or PDGF receptors may represent an effective strategy for treating KS.

Published

2005

3. Clonal selection for transcriptionally active viral oncogenes during progression to cancer.

Author

Van Tine BA, Kappes JC, Banerjee NS, Knops J, Lai L, Steenbergen RD, Meijer CL, Snijders PJ, Chatis P, Broker TR, Moen PT Jr, and Chow LT

Subjects

Cell Line, Transformed, Cell Nucleolus virology, DNA, Viral analysis, Humans, In Situ Hybridization, Fluorescence, Keratinocytes virology, Oncogene Proteins, Viral genetics, Papillomaviridae genetics, RNA, Viral genetics, RNA, Viral metabolism, Tyramine, Virus Integration, Cell Transformation, Neoplastic, Gene Expression Regulation, Viral, Oncogene Proteins, Viral metabolism, Papillomaviridae pathogenicity, Selection, Genetic, Transcription, Genetic

Abstract

Primary keratinocytes immortalized by human papillomaviruses (HPVs), along with HPV-induced cervical carcinoma cell lines, are excellent models for investigating neoplastic progression to cancer. By simultaneously visualizing viral DNA and nascent viral transcripts in interphase nuclei, we demonstrated for the first time a selection for a single dominant papillomavirus transcription center or domain (PVTD) independent of integrated viral DNA copy numbers or loci. The PVTD did not associate with several known subnuclear addresses but was almost always perinucleolar. Silent copies of the viral genome were activated by growth in the DNA methylation inhibitor 5-azacytidine. HPV-immortalized keratinocytes supertransduced with HPV oncogenes and selected for marker gene coexpression underwent crisis, and the surviving cells transcribed only the newly introduced genes. Thus, transcriptional selection in response to environmental changes is a dynamic process to achieve optimal gene expression for cell survival. This phenomenon may be critical in clonal selection during carcinogenesis. Examination of HPV-associated cancers supports this hypothesis.

Published

2004

4. Directly labeled mRNA produces highly precise and unbiased differential gene expression data.

Author

Gupta V, Cherkassky A, Chatis P, Joseph R, Johnson AL, Broadbent J, Erickson T, and DiMeo J

Subjects

Carbocyanines chemistry, DNA, Complementary genetics, Fluorescent Dyes chemistry, Gene Expression Profiling standards, HL-60 Cells, Humans, Jurkat Cells, Oligonucleotide Array Sequence Analysis methods, Oligonucleotide Array Sequence Analysis standards, RNA, Messenger chemistry, RNA, Messenger metabolism, Reproducibility of Results, Sensitivity and Specificity, Gene Expression Profiling methods, RNA, Messenger genetics

Abstract

Microarray based gene expression studies allow simultaneous analysis of relative amounts of messenger RNA (mRNA) for thousands of genes using fluorescently labeled nucleic acid targets. Most common methods use enzymatic techniques, such as oligo-dT primed reverse transcription to produce labeled cDNA. These labeling methods have a number of shortcomings, including enzyme- introduced labeling and sequence bias, laborious protocols, high experiment-to-experiment variability and an inability to detect small changes in expression levels. Here, we describe a novel labeling methodology that uses platinum-linked cyanine dyes to directly chemically label mRNA from as little as 2 micro g of total RNA. We show that the gene expression data produced using the labeled mRNA method has very high precision, low error, no labeling bias and a dynamic range over several orders of magnitude. This allows a greater accuracy in the identification of differentially expressed genes and cuts down on the need for running too many replicate assays. Small changes in gene expression can now be detected in large-scale gene expression profiling assays using this simple, easy and quick procedure.

Published

2003

5. Detection of viral RNA in CD4(-)CD8(-) and CD4(-)CD8(+) lymphocytes in vivo in rhesus monkeys infected with simian immunodeficiency virus of macaques.

Author

Huete JM, Chatis PA, Schmitz JE, Kuroda MJ, Letvin NL, and Reimann KA

Subjects

Animals, Cell Line, Transformed, Disease Models, Animal, Flow Cytometry, HIV Infections immunology, HIV Infections virology, Humans, Immunophenotyping, In Situ Hybridization, Fluorescence methods, Macaca mulatta, Simian Acquired Immunodeficiency Syndrome immunology, CD4-Positive T-Lymphocytes virology, CD8-Positive T-Lymphocytes virology, RNA, Viral blood, Simian Acquired Immunodeficiency Syndrome virology, Simian Immunodeficiency Virus isolation & purification

Abstract

A definition of the specific cell types that support HIV replication early in the course of infection will be important for understanding AIDS pathogenesis and designing strategies for preventing infection. Observations have indicated that the population of lymphocytes susceptible to productive infection extends beyond activated CD4(+) T cells. To explore this issue, we have employed laser scanning cytometry technology and the techniques of lymphocyte surface immunophenotyping followed by fluorescent in situ hybridization to detect simian immunodeficiency virus of macaques (SIVmac) RNA in phenotypically defined rhesus monkey lymphocytes. The immunophenotype of productively infected cells in either a rhesus monkey T cell line or in PBMCs infected in vitro with SIVmac was remarkably similar to that observed in productively infected PBMCs obtained from monkeys during primary infection. We observed low levels or no detectable expression of CD4 on cells infected in vitro or on PBMCs of infected monkeys. However, a substantial number of SIVmac-infected PBMCs both in cultured lymphocytes and sampled directly from infected monkeys expressed CD8 but not CD4. These observations are consistent with the possibility that the CD4 molecule may be modulated off the surface of CD4(+)CD8(-) or CD4(+)CD8(+) lymphocytes after infection or that infection occurred via a CD4-independent mechanism. Moreover, there was no preferential expression of CD25 on cells positive for SIVmac RNA, which might have been predicted if replication of the virus was occurring selectively in activated lymphocytes. These results broaden the range of lymphocytes that support productive SIVmac infection to include CD4(-)CD8(-) and CD4(-)CD8(+) subsets, and are consistent with virus replication occurring in nonactivated cells.

Published

2001

6. Efficient persistence of extrachromosomal KSHV DNA mediated by latency-associated nuclear antigen.

Author

Ballestas ME, Chatis PA, and Kaye KM

Subjects

Antigens, Viral analysis, Antigens, Viral genetics, Antigens, Viral metabolism, Cell Nucleus chemistry, Chromosomes chemistry, Cosmids, DNA, Viral analysis, DNA, Viral genetics, Herpesvirus 8, Human physiology, Humans, Interphase, Lymphocytes chemistry, Microscopy, Confocal, Nuclear Proteins analysis, Nuclear Proteins genetics, Transfection, Tumor Cells, Cultured, Chromosomes metabolism, DNA, Viral metabolism, Herpesvirus 8, Human genetics, Mitosis, Nuclear Proteins metabolism, Plasmids

Abstract

Primary effusion lymphoma (PEL) cells harbor Kaposi's sarcoma-associated herpesvirus (KSHV) episomes and express a KSHV-encoded latency-associated nuclear antigen (LANA). In PEL cells, LANA and KSHV DNA colocalized in dots in interphase nuclei and along mitotic chromosomes. In the absence of KSHV DNA, LANA was diffusely distributed in the nucleus or on mitotic chromosomes. In lymphoblasts, LANA was necessary and sufficient for the persistence of episomes containing a specific KSHV DNA fragment. Furthermore, LANA colocalized with the artificial KSHV DNA episomes in nuclei and along mitotic chromosomes. These results support a model in which LANA tethers KSHV DNA to chromosomes during mitosis to enable the efficient segregation of KSHV episomes to progeny cells.

Published

1999

7. Correlation of ribonucleic acid polymerase chain reaction, acid dissociated p24 antigen, and neopterin with progression of disease. A retrospective, longitudinal study of vertically acquired human immunodeficiency virus type 1 infection in children.

Author

Zaknun D, Orav J, Kornegay J, al-Attar I, Fuchs D, Zaknun J, Wachter H, Chatis P, Burchett SK, and McIntosh K

Subjects

Acquired Immunodeficiency Syndrome drug therapy, Anti-HIV Agents therapeutic use, Biopterins analogs & derivatives, Biopterins blood, CD4 Lymphocyte Count, Child, Child, Preschool, Female, Humans, Infant, Longitudinal Studies, Male, Neopterin, Retrospective Studies, Viral Load, Zalcitabine therapeutic use, Zidovudine therapeutic use, Acquired Immunodeficiency Syndrome virology, HIV Core Protein p24, HIV-1, Polymerase Chain Reaction, RNA, Viral

Abstract

Objective: We investigated the relationship between cell-free viral load, neopterin, age-adjusted CD4+ cell concentration, and clinical events in 49 children with vertically acquired human immunodeficiency virus type 1 infection., Study Design: Viral load was measured by quantitating viral ribonucleic acid in serum by polymerase chain reaction and measurement of immune complex dissociated p24 antigen in serum and plasma. Children were followed for an average of 2 1/2 years, with an average of 6 samples per child. Medical records were reviewed for weight, CD4+ cell count and clinical events., Results: High virus copy number in serum was predictive of a decrease in weight-for-age zscore during the subsequent 6 months. High viral load, low CD4+ cell count, and high neopterin level were correlated with encephalopathy. High viral load correlated with opportunistic infections. All of these relationships held regardless of treatment status, although viral load decreased significantly after treatment was begun., Conclusions: Measurements of viral load were useful prognostic indicators for poor weight gain. Elevated serum virus levels and neopterin values and low CD4+ cell counts were all associated with encephalopathy.

Published

1997

8. Age- and time-related changes in extracellular viral load in children vertically infected by human immunodeficiency virus.

Author

McIntosh K, Shevitz A, Zaknun D, Kornegay J, Chatis P, Karthas N, and Burchett SK

Subjects

Adult, Age Distribution, Child, Child, Preschool, Cohort Studies, Enzyme-Linked Immunosorbent Assay, Female, HIV pathogenicity, HIV Core Protein p24 blood, Humans, Incidence, Infant, Infectious Disease Transmission, Vertical, Linear Models, Male, Polymerase Chain Reaction, Prognosis, RNA, Viral blood, Retrospective Studies, Sampling Studies, Survival Rate, Time Factors, HIV immunology, HIV Core Protein p24 analysis, HIV Infections immunology, HIV Infections transmission, HIV Seropositivity epidemiology, RNA, Viral analysis

Abstract

Background: It is known that plasma or serum viral load is high in vertically HIV-infected children during the first year of life, but the changes in these titers after the first birthday have not been described. Information on the natural history of circulating extracellular virus will be useful in elucidating the pathogenesis of pediatric HIV infection and in using viral load measurement to guide prognosis and therapy., Methods: We measured serum RNA by reverse transcriptase-polymerase chain reaction and immune complex-dissociated p24 antigen enzyme-linked immunosorbent assay over time in 48 unselected children followed in our clinics and analyzed the findings in relation to age and clinical outcome., Results: In first-available samples from the 48 children there was a gradual reduction in HIV RNA values with increasing age, with a slope of -0.21 log copy/ml/year (P < 0.001, R2 = 0.6022). This downward trend was seen in subsets of children with all degrees of immunodeficiency. The mean slope of repeated HIV RNA measurements in individual children was similarly in a downward direction (slope -0.11 (P = 0.007 for difference from zero)). The slope was more negative in children who were younger at baseline. Immune complex-dissociated p24 antigen values were much less predictable and predictive., Conclusions: Viral load in vertically infected children, measured by reverse transcriptase-polymerase chain reaction, falls very gradually over time, descending from very high titers at the end of the first year, and reaching values seen in horizontally infected adults at approximately 5 years of age.

Published

1996

9. Determination of HIV-1 susceptibility to reverse transcriptase (RT) inhibitors by a quantitative cell-free RT assay.

Author

Greene RA, Japour AJ, Brewster F, Joseph RA, Chung PH, Kasila PA, and Chatis PA

Subjects

Cell-Free System, Drug Resistance, HIV-1 drug effects, Humans, Reproducibility of Results, Sensitivity and Specificity, Zidovudine pharmacology, Didanosine pharmacology, HIV Reverse Transcriptase antagonists & inhibitors, HIV-1 enzymology, Reverse Transcriptase Inhibitors pharmacology

Abstract

Background: Mutations in the human immunodeficiency virus type 1 (HIV-1) reverse transcriptase (RT) gene confer resistance to antiviral drugs acting on RT. Current methods employed to detect such resistance require time-consuming culture techniques during which selective pressures may affect the outcome of the test., Objectives: We sought to determine whether drug-susceptible and drug-resistant HIV-1 derived from clinical specimens could be distinguished by the effects of the active form of the drug on the enzyme activity in a quantitative, cell-free RT assay., Study Design: Polyethylene glycol (PEG)-precipitated virus was obtained from 7-day culture supernatants. RT activity in the lysed viral extracts was measured in the presence of increasing concentrations of the active form of the drug being tested. IC50 (50% inhibitory concentration) values were determined by application of the median effect equation., Results: Assays from nine post-nevirapine therapy isolates gave IC50 values at least 2 logs greater than pre-nevirapine isolates. The method also correctly distinguished between isolates sensitive and resistant to 2',3'-dideoxyinosine (ddI), but not between the ZDV-sensitive and ZDV-resistant isolates tested. The results agreed with data obtained by sequencing and by culture-based susceptibility assays.

Published

1996

10. AZT-related mutation Lys70Arg in reverse transcriptase of human immunodeficiency virus type 1 confers decrease in susceptibility to ddATP in in vitro RT inhibition assay.

Author

Sharma PL, Chatis PA, Dogon AL, Mayers DL, McCutchan FE, Page C, and Crumpacker CS

Subjects

Base Sequence, Didanosine therapeutic use, Humans, Molecular Sequence Data, Mutagenesis, Site-Directed, Polymerase Chain Reaction, Proviruses genetics, Reverse Transcriptase Inhibitors metabolism, Drug Resistance, Microbial genetics, HIV Infections drug therapy, HIV Infections genetics, HIV Reverse Transcriptase genetics, HIV-1 genetics, Zidovudine therapeutic use

Abstract

The genetic basis for didanosine (ddl) resistance in human immunodeficiency virus (HIV-1) has previously been shown to be commonly associated with a Leu to Val change at codon 74 in the HIV-1 RT gene. In this study sequential viral isolates were analyzed from five patients with prior zidovudine (AZT) use who received 6 to 16 months of ddl therapy. Following ddl therapy, viral isolates exhibited an increased AZT susceptibility and decreased ddl susceptibility. Sequence and nested PCR analysis of the HIV-1 RT gene revealed that two viral isolates contained the Leu to Val change at codon 74, and three other isolates with reduced susceptibility to ddl each contained changes at codons 65, 70, and 72. Site-directed mutagenesis was employed to insert specific mutations in RT gene of proviral clone pNL4-3. Analysis of virion-associated reverse transcriptase activity indicated that the Lys70Arg mutation resulted in an enzyme with 2- to 4-fold decreased susceptibility to ddATP. Statistical analysis of the inhibitory concentration for RT activity between pNL4-3 and mutant Lys70Arg viruses obtained in three independent RT inhibition assays was significant (P = 0.05) by student t test paired analysis. Drug susceptibility assays on the virus with Lys70Arg mutation showed a marginal decrease in susceptibility to ddl (1.5- to 2-fold) and about 4- to 6-fold decrease in susceptibility to AZT. Mutations Lys65Glu and Arg72Ser resulted in an impaired RT with greatly diminished functional RT activity. The AZT-associated Lys70Arg mutation results in an RT enzyme with decreased susceptibility to ddATP.

Published

1996

11. Human immunodeficiency virus type 1 entry into murine cell lines and lymphocytes from transgenic mice expressing a glycoprotein 120-binding mutant mouse CD4.

Author

Wieder KJ, Chatis P, Boltax J, Wieder I, Nuovo G, and Strom TB

Subjects

Amino Acid Sequence, Animals, CD4 Antigens genetics, Cell Line, Flow Cytometry, Humans, Mice, Mice, Transgenic, Molecular Sequence Data, Mutagenesis, Site-Directed, Mutation, Transfection, Virus Replication, CD4 Antigens metabolism, HIV Envelope Protein gp120 metabolism, HIV-1 physiology

Abstract

Human CD4, the receptor for the gp120 envelope glycoprotein of HIV-1, is the route for viral entry into CD4+ cells; other cellular factors may cooperate with CD4 to facilitate HIV-1 entry into human cells. Human CD4 expressed on murine cells does not readily mediate HIV-1 entry, which may reflect a functional incompatibility of human CD4 with murine cellular components. We postulated that a HIV-1 gp120-binding mutant murine CD4 (L3T4) possessing a minimal number of human amino acid residues could facilitate HIV-1 entry into rodent cells, unlike human CD4. This hypothesis led us to develop a series of murine L3T4 mutants that bear human CD4 gp120-binding region amino acid residues while retaining most L3T4 epitopes. HeLa cell transfectants expressing gp120-binding mutant L3T4 proteins could be infected with HIV-1. Three mouse cell lines expressing these L3T4 mutant proteins could also be infected with HIV-1 as determined by PCR techniques that detect viral DNA and spliced RNAs. Lectin-stimulated polymorphonuclear leukocytes from transgenic mice (SBL mouse) expressing a gp120-binding L3T4 mutant protein were infected with HIV-1 at the same frequency as lectin-stimulated human peripheral blood lymphocytes as determined by in situ PCR analyses. Supernatant p24gag and reverse transcriptase levels in HIV-infected mouse cell cultures, however, were routinely at background levels, unlike HIV-infected human cell cultures. Thus, gp120-binding mutant L3T4 proteins mediate viral entry in all mouse cells that were tested, but high-level viral replication is absent in these cells.

Published

1996

12. Concentrations of adipsin in blood and rates of adipsin secretion by adipose tissue in humans with normal, elevated and diminished adipose tissue mass.

Author

Napolitano A, Lowell BB, Damm D, Leibel RL, Ravussin E, Jimerson DC, Lesem MD, Van Dyke DC, Daly PA, and Chatis P

Subjects

Adolescent, Adult, Body Mass Index, Complement Factor D, Fasting, Female, Humans, Indians, North American, Insulin blood, Male, Reference Values, Sex Characteristics, Adipose Tissue metabolism, Body Composition, Obesity physiopathology, Serine Endopeptidases blood, Serine Endopeptidases metabolism

Abstract

Adipsin, which is identical to complement factor D, is synthesized by fat cells, circulates in the bloodstream and is profoundly deficient in mice with genetic and hypothalamic obesity. With the recent cloning of human adipsin, a quantitative human immunoassay has been developed. In the present study, we measured adipsin blood concentrations in humans with increased and decreased adipose stores as well as adipsin secretion by adipose tissue obtained from lean and obese individuals. The results demonstrate that adipsin is released by human adipose tissue fragments as has previously been shown in mice, and that, in contrast to obese mice, blood adipsin concentrations were not reduced in the obese humans tested in this study. We also observed that blood adipsin concentrations can vary as a function of feeding or adiposity, in that they tend to be mildly elevated in obese individuals or mildly reduced in individuals with total lipo-atrophy, cachexia related to AIDS and anorexia nervosa. Thus, the circulating concentration of adipsin tends to correlate positively with degree of adiposity. Clearly, no deficiency in blood adipsin concentrations or adipsin secretion by adipose tissue was observed in the obese individuals studied.

Published

1994

13. Cytomegalovirus infection of the BS-1 human stroma cell line: effect on murine hemopoiesis.

Author

Steinberg HN, Anderson J Jr, Lim B, and Chatis PA

Subjects

Animals, Cell Line, Culture Techniques methods, Humans, Mice, Mice, Inbred C57BL, Bone Marrow microbiology, Cytomegalovirus growth & development, Hematopoiesis physiology, Hematopoietic Stem Cells microbiology, Stromal Cells microbiology

Abstract

BS-1, a stromal cell line derived from human bone marrow, can support the growth of murine erythroid (BFU-E), granulocyte-macrophage (CFU-GM), and megakaryocyte (CFU-M) progenitor cells in a short term in vitro coculture system. Exposure of BS-1 cells to cytomegalovirus (CMV) for 3 hr prior to coculture results in a marked reduction in the stroma cell's ability to support murine hemopoiesis. CMV's effect on the BS-1 cell's hematopoietic support function is dependent on the multiplicity of infection with total suppression of BFU-E observed at a 1:1 ratio of virus to bone marrow cells. A 50% loss in the ability of BS-1 cells to support BFU-E is observed at a 0.1:1 ratio. No effect of CMV is observed with further log dilutions of virus. CMV infection of BS-1 cells affects its support of erythroid progenitor cell growth to a greater extent than its influence on the development of granulocyte-macrophage colonies. Antibody to CMV or heat inactivation of the virus reverses the inhibitory affect on BS-1 cells. The results suggest that CMV can infect a cell that constitutes one of the cellular elements of the normal bone marrow microenvironment causing a decrease in the stroma's ability to support the growth and development of normal progenitor cells.

Published

1993

14. HIV infection of the BS-1 human stroma cell line: effect on murine hematopoiesis.

Author

Steinberg HN, Anderson J, Crumpacker CS, and Chatis PA

Subjects

Animals, Cell Communication physiology, Cell Division physiology, Cells, Cultured, Humans, Mice, Stromal Cells physiology, HIV physiology, Hematopoiesis physiology, Hematopoietic Stem Cells physiology, Stromal Cells microbiology

Abstract

BS-1, a stroma cell line derived from normal human bone marrow, can support the growth of murine erythroid (BFU-E), granulocyte-macrophage (CFU-GM), and megakaryocyte (CFU-Meg) progenitor cells in a short-term in vitro coculture system. Exposure of BS-1 cell to the human immunodeficiency virus (HIV) prior to coculture results in a marked reduction in the stroma cell's ability to support murine BFU-E and CFU-GM. The effect of HIV on the BS-1 cell's hematopoietic support function (HSF) is dependent on the multiplicity of infection (m.o.i.). BS-1 stimulation of CFU-GM is significantly impaired at m.o.i. values ranging from 10 to 0.1, whereas its support of BFU-E colony formation is inhibited at m.o.i. values of 10 and 1. No effect of HIV on the BS-1 cell's HSF is observed with further log dilutions of virus. The HIV-mediated suppression of the BS-1 cell's ability to support hematopoiesis is neutralized by a monoclonal antibody (titers ranging from 1:10 to 1:50) to the Gp160 surface antigen of the virus. Suppression of BS-1 cell's HSF is again observed with log dilution (> 1:100) of the antibody. HIV suppression of the BS-1 cell's HSF correlates with replication of the virus. P24 antigen levels of 150 pG/ml are measured as early as Day 6 postinfection and rise to 360 pG/ml by Day 16 of culture. The results suggest that HIV may impair normal hematopoiesis by infecting the stroma cells of the bone marrow microenvironment and compromising their role as accessory cells in supporting the proliferation and differentiation of hematopoietic progenitor cells.

Published

1993

15. Resistance of herpesviruses to antiviral drugs.

Author

Chatis PA and Crumpacker CS

Subjects

Drug Resistance, Microbial, Antiviral Agents pharmacology, Herpesviridae drug effects

Published

1992

16. A controlled trial comparing foscarnet with vidarabine for acyclovir-resistant mucocutaneous herpes simplex in the acquired immunodeficiency syndrome. The AIDS Clinical Trials Group.

Author

Safrin S, Crumpacker C, Chatis P, Davis R, Hafner R, Rush J, Kessler HA, Landry B, and Mills J

Subjects

Acyclovir pharmacology, Adult, Antiviral Agents administration & dosage, Drug Resistance, Microbial, Female, Foscarnet, Humans, Male, Phosphonoacetic Acid administration & dosage, Phosphonoacetic Acid adverse effects, Phosphonoacetic Acid therapeutic use, Recurrence, Simplexvirus drug effects, Vidarabine administration & dosage, Vidarabine adverse effects, Acquired Immunodeficiency Syndrome complications, Antiviral Agents therapeutic use, Herpes Genitalis drug therapy, Phosphonoacetic Acid analogs & derivatives, Stomatitis, Herpetic drug therapy, Vidarabine therapeutic use

Abstract

Background and Methods: Most strains of herpes simplex virus that are resistant to acyclovir are susceptible in vitro to both foscarnet and vidarabine. We conducted a randomized trial to compare foscarnet with vidarabine in 14 patients with the acquired immunodeficiency syndrome (AIDS) and mucocutaneous herpetic lesions that had been unresponsive to intravenous therapy with acyclovir for a minimum of 10 days. The patients were randomly assigned to receive either foscarnet (40 mg per kilogram of body weight intravenously every 8 hours) or vidarabine (15 mg per kilogram per day intravenously) for 10 to 42 days. In the isolates of herpes simplex virus we documented in vitro resistance to acyclovir and susceptibility to foscarnet and vidarabine., Results: The lesions in all eight patients assigned to foscarnet healed completely after 10 to 24 days of therapy. In contrast, vidarabine was discontinued because of failure in all six patients assigned to receive it. The time to complete healing (P = 0.01), time to 50 percent reductions in the size of the lesions (P = 0.01) and the pain score (P = 0.004), and time to the end of viral shedding (P = 0.006) were all significantly shorter in the patients assigned to foscarnet. Three patients had new neurologic abnormalities while receiving vidarabine. No patient discontinued foscarnet because of toxicity. Although initial recurrences of herpes simplex infection after the index lesion had healed tended to be susceptible to acyclovir, acyclovir-resistant infection eventually recurred in every healed patient, a median of 42.5 days (range, 14 to 191) after foscarnet was discontinued., Conclusions: For the treatment of acyclovir-resistant herpes simplex infection in patients with AIDS, foscarnet has superior efficacy and less frequent serious toxicity than vidarabine. Once the treatment is stopped, however; there is a high frequency of relapse.

Published

1991

17. Detection of human immunodeficiency virus type 1 clinical isolates with reduced sensitivity to zidovudine and dideoxyinosine by RNA.RNA hybridization.

Author

Japour AJ, Chatis PA, Eigenrauch HA, and Crumpacker CS

Subjects

Cloning, Molecular, HIV-1 growth & development, Humans, In Vitro Techniques, Leukocytes, Mononuclear microbiology, Microbial Sensitivity Tests, Nucleic Acid Hybridization, RNA Probes, RNA-Directed DNA Polymerase genetics, Reverse Transcriptase Inhibitors, Sequence Homology, Nucleic Acid, Didanosine administration & dosage, HIV-1 drug effects, RNA, Viral analysis, Zidovudine administration & dosage

Abstract

A quantitative rapid assay to detect resistant clinical human immunodeficiency virus type 1 (HIV-1) strains remains an important medical goal. A system incorporating a quantitative RNA.RNA hybridization assay that measures the amount of intracellular HIV-1-specific RNA has been employed to detect the level of inhibition by nucleoside analogues in sensitive and resistant HIV-1 strains. The RNA.RNA hybridization assay readily distinguished previously published zidovudine (ZDV; 3'-azido-3'-deoxythymidine)-resistant isolates from ZDV-sensitive isolates of HIV-1. The 50% inhibitory concentration (IC50) of ZDV for HTLV-IIIB and sensitive clinical HIV-1 isolates is between 0.01 and 0.04 microM. HIV-1 strains from three patients on long-term ZDV therapy displayed a greater than 20-fold increase in the ZDV IC50 compared to sensitive strains. The drug sensitivity system was confirmed by showing that mutations in the HIV reverse transcriptase gene from a ZDV-resistant isolate resulted in four amino acid changes (Leu-125----Trp, Ile-142----Val, Thr-215----Tyr, and Pro-294----Thr) including one change (Thr-215----Tyr) that has been previously reported to be associated with resistance. One clinical HIV strain with high-level ZDV resistance displayed a 5-fold increase in 2',3'-dideoxyinosine IC50 compared to that of HTLV-IIIB. A drug sensitivity assay employing RNA.RNA hybridization may be useful for extensive screening of HIV isolates from patients enrolled in clinical trials and permit the correlation of in vitro resistance with clinical outcome.

Published

1991

18. In vitro suppression of normal human bone marrow progenitor cells by human immunodeficiency virus.

Author

Steinberg HN, Crumpacker CS, and Chatis PA

Subjects

Bone Marrow microbiology, Cell Division, Colony-Forming Units Assay, DNA Probes, Gene Products, env immunology, HIV immunology, HIV Envelope Protein gp160, Hematopoietic Stem Cells physiology, Humans, In Vitro Techniques, Leukocyte Count, Polymerase Chain Reaction, Protein Precursors immunology, T-Lymphocyte Subsets microbiology, Virus Replication, HIV physiology, HIV Infections microbiology, Hematopoietic Stem Cells microbiology

Abstract

Incubation of normal human nonadherent and T-cell-depleted bone marrow cells with HIVIIIB at multiplicities of infection (MOI) ranging from 0.0001:1 to 1:1 reverse transcriptase (RT) units resulted in the dose-dependent suppression of the in vitro growth of erythroid burst-forming unit (BFU-E), granulocyte-macrophage (CFU-GM), and T-lymphocyte (CFU-TL) colonies of progenitor cells. Maximum inhibition of colony formation was observed at a 1:1 ratio of virus to bone marrow cells. At this MOI, BFU-E and CFU-GM colonies were inhibited by 60 to 80%, while CFU-TL colonies were totally suppressed. Inhibition of colony formation was also observed at an MOI of 0.1:1 but not with further log dilutions of the virus. Incubation of the virus with antibody to gp160 resulted in the complete reversal of stem cell suppression and the normalization of colony growth in vitro. For BFU-E and CFU-GM colonies, this reversal was observed with dilutions of antibody up to 1:100 and was no longer observed at titers greater than 1:500. The CFU-TL colony number normalized at titers between 1:10 and 1:50. Human immunodeficiency virus (HIV) also suppressed by 50% the growth of colonies derived from CD34+ stem cell fractions. Infection of CD34+ cells and T-cell-depleted, nonadherent cell fractions was demonstrated by detection with HIV-specific DNA probe following amplification by polymerase chain reaction. The results suggest that HIV can directly infect human bone marrow progenitor cells and affect their ability to proliferate and give rise to colonies in vitro. The results indicate a direct role for the virus in bone marrow suppression and a possible mechanism for the cytopenias observed in patients with AIDS.

Published

1991

19. Analysis of the thymidine kinase gene from clinically isolated acyclovir-resistant herpes simplex viruses.

Author

Chatis PA and Crumpacker CS

Subjects

Acquired Immunodeficiency Syndrome complications, Acquired Immunodeficiency Syndrome microbiology, Drug Resistance, Microbial genetics, Humans, Simplexvirus drug effects, Simplexvirus isolation & purification, Viral Plaque Assay, Acyclovir pharmacology, Genes, Viral, Simplexvirus genetics, Thymidine Kinase genetics, Viral Structural Proteins genetics

Abstract

The isolation and description of acyclovir-resistant (ACVR) herpes simplex-2 viruses from patients with AIDS has recently been reported. These ACVR viruses were all markedly decreased in their thymidine kinase (TK) activity, and 6 of 10 of these TK viruses were able to establish latency. In addition, one of these isolates, ACVR-86012 was neuropathogenic in a murine encephalitis model. In this paper, the characteristics of these isolates with respect to TK polypeptide synthesis are examined. All but one isolate synthesized a detectable TK protein by immunoprecipitation, and 9/10 of the TK proteins had an altered electrophoretic mobility as compared to wild-type. The TK polypeptide from the neuropathogenic isolate ACVR-86012 was full-length and the gene was sequenced. An amino acid change from a glutamine to a proline at amino acid residue 105 was detected compared to the wild-type HSV-333 strain. These results indicate that an amino acid change in the NH2 portion of the TK protein is associated with a full-length peptide with decreased enzyme activity but the virus retains neuropathic virulence.

Published

1991

20. Construction of recombinants between molecular clones of murine retrovirus MCF 247 and Akv: determinant of an in vitro host range property that maps in the long terminal repeat.

Author

Holland CA, Wozney J, Chatis PA, Hopkins N, and Hartley JW

Subjects

Animals, Base Sequence, DNA Restriction Enzymes, Genes, Mice, Mice, Inbred Strains, Species Specificity, Transfection, Cloning, Molecular, DNA, Recombinant metabolism, Genes, Viral, Leukemia Virus, Murine genetics, Viral Proteins genetics

Abstract

The leukemogenic mink cell focus-forming (MCF) retroviruses such as MCF 247 have biological properties distinct from those of their ecotropic progenitors. Nucleotide sequences encoding portions of gp70, Prp15E, and the long terminal repeat differ between the two types of viruses. To investigate the role of each of these genetic elements in determining the biological properties of MCF viruses, we prepared infectious molecular clones of MCF 247 and generated a set of recombinants between these clones and a molecular clone of Akv, the ecotropic parent of MCF 247. Each molecular clone of MCF 247 was distinct. All the recombinants between Akv and MCF 247 yielded infectious virus upon transfection. Most interestingly, recombinants which contain the long terminal repeat of MCF 247 were found to have an in vitro host range property that has been correlated with high oncogenic activity and thymotropism of certain MCF isolates; namely, they plated with higher efficiency on SC-1 cells than on NFS mouse embryo cells. Nononcogenic MCF isolates showed a slight preference for NFS cells, whereas Akv virus plated with approximately equal efficiency on the two cell types.

Published

1985

21. Acyclovir-resistant herpes simplex virus infections in patients with the acquired immunodeficiency syndrome.

Author

Erlich KS, Mills J, Chatis P, Mertz GJ, Busch DF, Follansbee SE, Grant RM, and Crumpacker CS

Subjects

Adult, Animals, Drug Resistance, Microbial, Encephalitis etiology, Humans, Male, Mice, Mice, Inbred BALB C, Microbial Sensitivity Tests, Simplexvirus isolation & purification, Simplexvirus pathogenicity, Thymidine Kinase analysis, Virulence, Acquired Immunodeficiency Syndrome complications, Acyclovir pharmacology, Herpes Simplex microbiology, Simplexvirus drug effects

Published

1989

22. Characterization of the soluble glycoprotein released from vesicular stomatitis virus-infected cells.

Author

Chatis PA and Morrison TG

Subjects

Animals, Cell Line, Cricetinae, Female, Glycoproteins analysis, Isoelectric Point, Molecular Weight, Mutation, Peptides analysis, Temperature, Tunicamycin pharmacology, Viral Proteins analysis, Cell Membrane metabolism, Glycoproteins metabolism, Vesicular stomatitis Indiana virus metabolism, Viral Proteins metabolism

Abstract

Vesicular stomatitis virus-infected Chinese hamster ovary cells release into the extracellular medium a soluble form of the vesicular stomatitis virus glycoprotein (G protein) termed Gs (Kang and Prevec, Virology 46:678-680, 1971). The properties of this molecule and the cellular site at which it is generated were characterized. By comparing the sizes and the peptide maps of the unglycosylated forms of G and Gs, we found that between 5,000 and 6,000 daltons of the carboxy-terminal end of the G protein is cleaved to generate the Gs molecule. This truncated molecule contains no fatty acid. Gs released from cells grown at 39 degrees C migrated on polyacrylamide gels slightly slower than Gs released at 30 degrees C. The unglycosylated form of Gs also showed this size difference. Furthermore, unglycosylated Gs was resolved into two species upon isoelectric focusing: the relative amounts of the two species depended upon the temperature at which infected cells were incubated. Full-sized unglycosylated virus-associated G also was resolved into two species, but the more basic form predominated at both 30 and 39 degrees C. The appearance of Gs in the extracellular medium depended upon the presence of stable, full-sized G at the cell surface. The amount of Gs released was quantitated in seven different situations in which the migration of G to the cell surface was inhibited. In all cases, the amount of Gs released was also decreased. In addition, incubation of cells surface labeled with 125I resulted in the release of 125I-labeled Gs protein, as well as full-sized G protein. These results suggest that Gs is generated primarily by proteolytic cleavage of plasma membrane-associated G at a site in the molecule just amino terminal to the membrane-spanning region of the molecule.

Published

1983

23. Role for the 3' end of the genome in determining disease specificity of Friend and Moloney murine leukemia viruses.

Author

Chatis PA, Holland CA, Hartley JW, Rowe WP, and Hopkins N

Subjects

Animals, Cells, Cultured, DNA Restriction Enzymes, DNA, Recombinant metabolism, Friend murine leukemia virus pathogenicity, Mice, Mice, Inbred BALB C, Mice, Inbred Strains, Moloney murine leukemia virus pathogenicity, Species Specificity, Transfection, Cloning, Molecular, Friend murine leukemia virus genetics, Genes, Viral, Leukemia, Experimental microbiology, Moloney murine leukemia virus genetics

Abstract

To probe the genetic basis of disease specificity of nondefective murine type C viruses, we are constructing recombinants in vitro between molecular clones of Friend murine leukemia virus (Fr-MuLV) and Moloney murine leukemia virus (Mo-MuLV). Fr-MuLV induces erythroleukemias when injected into newborn NFS mice, whereas Mo-MuLV almost invariably induces T-cell lymphomas. We find that a recombinant whose genome is derived primarily from Fr-MuLV but which has 621 nucleotides of Mo-MuLV information at its 3' end induces almost exclusively thymic lymphomas. The sequences derived from Mo-MuLV include 99 nucleotides encoding the carboxyl terminus of Prp15E, the origin of DNA +-strand synthesis, all of the U3 region, and 36 nucleotides of the R portion of the long terminal repeat. When the segment of Mo-MuLV was removed and replaced with the comparable segment from Fr-MuLV, the virus was again erythroblastosis-inducing. These results, in conjunction with studies from other laboratories [Laimins, L. A., Khoury, G., Gorman, C., Howard, B. & Gruss, P. (1982) Proc. Natl. Acad. Sci. USA 79, 6453-6457], suggest that transcriptional signals in U3 may determine tissue tropism and hence influence disease specificity ("targeting") of murine leukemia viruses.

Published

1983

24. A 3' end fragment encompassing the transcriptional enhancers of nondefective Friend virus confers erythroleukemogenicity on Moloney leukemia virus.

Author

Chatis PA, Holland CA, Silver JE, Frederickson TN, Hopkins N, and Hartley JW

Subjects

Animals, Base Sequence, Cells, Cultured, Cloning, Molecular, DNA Restriction Enzymes, DNA, Recombinant metabolism, Friend murine leukemia virus pathogenicity, Mice, Mice, Inbred Strains, Moloney murine leukemia virus pathogenicity, Plasmids, Cell Transformation, Neoplastic, Enhancer Elements, Genetic, Friend murine leukemia virus genetics, Genes, Regulator, Leukemia, Experimental microbiology, Moloney murine leukemia virus genetics

Abstract

Nondefective Friend helper murine leukemia virus (Fr-MuLV) induces primarily erythroleukemias in NFS mice, whereas Moloney murine leukemia virus (Mo-MuLV) induces T cell lymphomas. Using molecular clones of these two viruses, we constructed a recombinant in which a 0.62-kilobase fragment encompassing the U3 region at the 3' end of the Fr-MuLV genome replaced the corresponding region of Mo-MuLV. The recombinant virus obtained by transfection of this clone, whose genome is derived primarily from Mo-MuLV, induces almost exclusively erythroleukemias in NFS mice. This and the previous result of Chatis et al. (Proc. Natl. Acad. Sci. U.S.A. 80:4408-4411), showing that the reciprocal recombinant whose genome is primarily derived from Fr-MuLV induces almost exclusively lymphomas, argue that a strong determinant of the distinct disease specificities of Fr-MuLV and Mo-MuLV lies in this 3' end 0.62-kilobase fragment which contains the putative virus enhancers. To more precisely define this determinant, we have begun to construct recombinants in which smaller 3' end fragments of the Fr-MuLV and Mo-MuLV genomes are exchanged. Analysis of the first such recombinant showed that Fr-MuLV can be converted to a lymphoma-inducing virus in NFS mice by substitution of a 0.38-kilobase fragment encompassing the virus enhancers in U3 with the corresponding region of the Mo-MuLV genome.

Published

1984

25. Mutational changes in the vesicular stomatitis virus glycoprotein affect the requirement of carbohydrate in morphogenesis.

Author

Chatis PA and Morrison TG

Subjects

Glycoproteins metabolism, Morphogenesis, Temperature, Tunicamycin pharmacology, Vesicular stomatitis Indiana virus drug effects, Vesicular stomatitis Indiana virus metabolism, Viral Proteins metabolism, Virus Replication, Carbohydrate Metabolism, Glycoproteins genetics, Mutation, Vesicular stomatitis Indiana virus genetics, Viral Proteins genetics

Abstract

The role of carbohydrate in the morphogenesis of vesicular stomatitis virus was studied, using the antibiotic tunicamycin to inhibit glycosylation. It has been reported previously (Gibson et al., J. Biol. Chem. 254:3600-3607, 1979) that the San Juan strain of vesicular stomatitis virus requires carbohydrate for efficient migration of the glycoprotein (G) to the cell surface and for virion formation, whereas the prototype or Orsay strain of vesicular stomatitis virus is less stringent in its carbohydrate requirement at 30 degrees C. However, there are many differences between the two strains. We found that mutational changes within the G protein of the same strain of virus (prototype or Orsay) alters the requirement for carbohydrate at 30 degrees C. Group V or G protein mutants tsO45 and tsO44, like their prototype parent, did not require carbohydrate for efficient morphogenesis. In contrast, the G protein of another group V mutant, tsO110, was totally dependent upon carbohydrate addition for migration to the cell surface. Furthermore, no tsO110 particles were released in the absence of glycosylation. The wild-type prototype strain did require carbohydrate at 39.5 degrees C for insertion of the G protein into the plasma membrane and virion formation. However, a pseudorevertant of tsO44 (tsO44R), unlike the prototype parent, no longer exhibited this temperature-sensitive requirement for carbohydrate. At 39.5 degrees C in the presence of tunicamycin, tsO44R-infected cells released normal yields of particles and the unglycosylated G reached the cell surface very efficiently. In contrast to tsO110, which absolutely requires carbohydrate, mutational change in the tsO44R G protein has eliminated the requirement for carbohydrate. Thus, simple mutational changes, as opposed to many changes in the molecule, are sufficient to alter the carbohydrate requirement.

Published

1981

26. Functional expression of a cloned herpes simplex virus type 1 DNA polymerase gene.

Author

Dorsky D, Chatis P, and Crumpacker C

Subjects

Animals, Cell Line, Cloning, Molecular, Gene Expression Regulation, Genes, Viral, Genetic Complementation Test, Genetic Vectors, Recombinant Proteins genetics, DNA-Directed DNA Polymerase genetics, Simplexvirus genetics

Abstract

A vector which expresses the herpes simplex virus type 1 (HSV-1) (strain 17) DNA polymerase gene was constructed by ligating two separately cloned HSV DNA restriction fragments into an intermediate plasmid and then mobilizing the intact polymerase gene-encoding sequence into a pSV2 derivative. The expression vector (pD7) contains a functional simian virus 40 replication origin and early enhancer-promoter upstream from the HSV DNA polymerase-encoding sequence. COS-1 cells transfected with pD7 contained an RNA species, shown by Northern blot analysis to hybridize specifically with an HSV DNA pol probe and to be the same size (4.3 kilobases) as the pol mRNA found in HSV-1-infected COS-1 cells. A genetic complementation test was used to establish that pD7 expresses a functional pol gene product. COS-1 cells transfected with pD7 were able to partially complement the growth defect of an HSV-1 (KOS) temperature-sensitive mutant, tsC7, in the DNA polymerase gene at the nonpermissive temperature.

Published

1987

27. Successful treatment with foscarnet of an acyclovir-resistant mucocutaneous infection with herpes simplex virus in a patient with acquired immunodeficiency syndrome.

Author

Chatis PA, Miller CH, Schrager LE, and Crumpacker CS

Subjects

Adult, Drug Resistance, Microbial, Female, Foscarnet, Herpes Genitalis drug therapy, Humans, Phosphonoacetic Acid analogs & derivatives, Simplexvirus isolation & purification, Skin Diseases, Infectious drug therapy, Acquired Immunodeficiency Syndrome complications, Acyclovir pharmacology, Antiviral Agents therapeutic use, Herpes Simplex drug therapy, Organophosphorus Compounds therapeutic use, Phosphonoacetic Acid therapeutic use, Simplexvirus drug effects

Published

1989

28. Fatty acid modification of Newcastle disease virus glycoproteins.

Author

Chatis PA and Morrison TG

Subjects

Acylation, Animals, Cell Line, Chick Embryo, Cricetinae, Female, Hemagglutinins, Viral, Neuraminidase, Palmitic Acid, Glycoproteins metabolism, Newcastle disease virus metabolism, Palmitic Acids metabolism, Viral Proteins metabolism

Abstract

The fatty acid acylation of Newcastle disease virus hemagglutininin-neuraminidase and fusion glycoproteins was assayed. [3H]palmitate label was associated with cytoplasmic fusion proteins (F0 and F1) and virion-associated F1. In contrast, there was no detectable [3H]palmitate label associated with the hemagglutin-neuraminidase protein in Newcastle disease virus-infected Chinese hamster ovary cells or chicken embryo cells or in virions released from these cells. Thus, fatty acid modification may not be important for the maturation of some glycoproteins.

Published

1982

29. Vesicular stomatitis virus glycoprotein is anchored to intracellular membranes near its carboxyl end and is proteolytically cleaved at its amino terminus.

Author

Chatis PA and Morrison TG

Subjects

Cell Line, Chymotrypsin metabolism, Intracellular Membranes analysis, Methionine analysis, Peptides analysis, Trypsin metabolism, Glycoproteins analysis, Vesicular stomatitis Indiana virus analysis, Viral Proteins analysis

Abstract

The intracellular vesicular stomatitis virus glycoprotein (G) is inserted into membranes such that a small portion of one end of the molecule is exposed on the cytoplasmic surface of the endoplasmic reticulum and is susceptible to proteolytic digestion (T.G. Morrison, C.O. McQuain, and D. Simpson, J. Virol. 28:368-374). We have determined that this region of the G protein contains two methionyl tryptic peptides. The methionyl tryptic peptides of the G protein have been ordered by the use of the antibiotic pactamycin, and the two methionyl tryptic peptides removed by proteolytic digestion of intracellular G protein have been shown to be derived from the carboxyl terminal end of the protein. In addition, we have found that the unglycosylated G protein synthesized in a reticulocyte cell-free reaction migrates on polyacrylamide gels slightly slower than the unglycosylated G protein synthesized in tunicamycin-treated infected cells. We have also compared these G proteins derived from different sources by partial proteolysis (D.W. Cleveland, S.G. Fischer, M.W. Kirschner, and V.K. Laemmli, J. Biol. Chem. 252:1102-1106) and by chymotryptic peptide analysis. We have found minor differences between the two proteins consistent with the removal of 10 to 15 amino acids from the amino terminus of the intracellular G protein.

Published

1979