Your search keyword '"Susan Grimm"' showing total 11 results

1. Blessed Sacrament School Parking Lot: Friday Night

Author

Susan Grimm

Subjects

Parking lot, Advertising, General Medicine, Business

Published

2019

2. 2′-SUBSTITUTED PHOSPHOROTHIOATE CONTAINING OLIGORIBONUCLEOTIDES: AN APPLICATION TO THE SYNTHESIS AND PURIFICATION OF HAMMERHEAD RIBOZYMES

Author

Nassim Usman, Lara Maloney, Peter Haeberli, Anthony DiRenzo, Francine E. Wincott, Susan Grimm, and Kurt Levy

Subjects

Nuclease, biology, Ribozyme, RNA, Biochemistry, Combinatorial chemistry, Catalysis, chemistry.chemical_compound, chemistry, Ribose, Genetics, biology.protein, Oligoribonucleotides, Ligase ribozyme

Abstract

A systematic study of the catalytic activity and nuclease stability of selectively modified hammerhead ribozymes has resulted in the identification of a generic motif containing 5 ribose residues and 31 2′- modified sugars (1). This substructure has been further elaborated to include phosphorothioate linkages. Although oligodeoxyribonucleotides containing phosphorothioate linkages have been studied extensively, similarly substituted RNA molecules or ribozymes have not been explored at-length. The synthesis and purification of these ribozymes is discussed (2).

Published

1996

3. Crystal structures of an A-form duplex with single-adenosine bulges and a conformational basis for site-specific RNA self-cleavage

Author

Nassim Usman, Stefan Portmann, Susan Grimm, Christopher T. Workman, and Martin Egli

Subjects

Clinical Biochemistry, Stacking, Crystal structure, Crystallography, X-Ray, Biochemistry, Bulge, Drug Discovery, Molecule, Nucleotide, Structural motif, Molecular Biology, X-ray crystallography, Pharmacology, chemistry.chemical_classification, major and minor groove widths, RNA-Binding Proteins, RNA, General Medicine, bending, transesterification, Crystallography, chemistry, Duplex (building), Nucleic Acid Conformation, Molecular Medicine, base triples

Abstract

Background: Bulged nucleotides are common secondary structural motifs in RNA molecules and are often involved in RNA-RNA and RNA-protein interactions. RNA is selectively cleaved at bulge sites (when compared to other sites within stems) in the presence of divalent metal cations. The effects of bulge nucleotides on duplex stability and topology have been extensively investigated, but no detailed X-ray structures of bulge-containing RNA fragments have been available. Results: We have crystallized a self-complementary RNA-DNA chimeric 11-nucleotide sequence containing single-adenosine bulges under two different conditions, giving two distinct crystal forms. In both lattices the adenosines are looped out, leaving the stacking interactions in the duplex virtually unaffected. The bulges cause the duplex to kink in both cases. In one of the structures, the conformation of the bulged nucleotide places its modeled 2′-oxygen in line with the adjacent phosphate on the 3′ side, where it is poised for nucleophilic attack. Conclusions: Single adenosine bulges cause a marked opening of the normally narrow RNA major groove in both crystal structures, rendering the bases more accessible to interacting molecules compared with an intact stem. The geometries around the looped-out adenosines are different in the two crystal forms, indicating that bulges can confer considerable local plasticity on the usually rigid RNA double helix. The results provide a conformational basis for the preferential, metal-assisted self-cleavage of RNA at bulged sites.

Published

1996

4. Chemical Modification of Hammerhead Ribozymes

Author

Leonid Beigelman, Alexander Karpeisky, James McSwiggen, Varykina G. Thackray, Kristi Jensen, Francine E. Wincott, Nassim Usman, Jasenka Matulic-Adamic, Kenneth G. Draper, Danuta Tracz, David Sweedler, Anil S. Modak, Carolyn Gonzalez, Susan Grimm, Peter Haeberli, and Anthony DiRenzo

Subjects

chemistry.chemical_classification, Nuclease, biology, Ribozyme, Cell Biology, Biochemistry, Uridine, chemistry.chemical_compound, chemistry, biology.protein, Structure–activity relationship, Nucleotide, Mammalian CPEB3 ribozyme, Hairpin ribozyme, Molecular Biology, Ligase ribozyme

Abstract

A systematic study of selectively modified, 36-mer hammerhead ribozymes has resulted in the identification of a generic, catalytically active and nuclease stable ribozyme motif containing 5 ribose residues, 29-30 2'-O-Me nucleotides, 1-2 other 2'-modified nucleotides at positions U4 and U7, and a 3'-3'-linked nucleotide "cap." Eight 2'-modified uridine residues were introduced at positions U4 and U7. From the resulting set of ribozymes, several have almost wild-type catalytic activity and significantly improved stability. Specifically, ribozymes containing 2'-NH2 substitutions at U4 and U7, or 2'-C-allyl substitutions at U4, retain most of their catalytic activity when compared to the all-RNA parent. Their serum half-lives were 5-8 h in a variety of biological fluids, including human serum, while the all-RNA parent ribozyme exhibits a stability half-life of only approximately 0.1 min. The addition of a 3'-3'-linked nucleotide "cap" (inverted T) did not affect catalysis but increased the serum half-lives of these two ribozymes to > 260 h at nanomolar concentrations. This represents an overall increase in stability/activity of 53,000-80,000-fold compared to the all-RNA parent ribozyme.

Published

1995

5. Synthesis, deprotection, analysis and purification of RNA and ribosomes

Author

Francine Wincott, Anthony DiRenzo, Chris Shaffer, Susan Grimm, Danuta Tracz, Christopher Workman, David Sweedler, Carolyn Gonzalez, Stephen Scaringe, and Nassim Usman

Subjects

Molecular Sequence Data, Tetrazoles, RNA chemical synthesis, Hydrofluoric Acid, Methylamines, RNA analysis, Ethylamines, Methods, Genetics, RNA, Catalytic, Base sequence, Chromatography, High Pressure Liquid, chemistry.chemical_classification, Base Sequence, biology, Ion exchange, Ribozyme, RNA, Chromatography, Ion Exchange, Pyrrolidinones, Enzyme, chemistry, Biochemistry, biology.protein, Indicators and Reagents

Abstract

Improvements in the synthesis, deprotection and purification of oligoribonucleotides are described. These advances allow for reduced synthesis and deprotection times, while improving product yield. Coupling times are reduced by half using 5-ethylthio-1H-tetrazole (S-ethyltetrazole) as the activator. Base and 2'-O-t-butyldimethylsilyl deprotection with methylamine (MA) and anhydrous triethylamine/hydrogen fluoride in N-methylpyrrolidinone (TEA.HF/NMP), respectively, requires a fraction of the time necessitated by current standard methods. In addition, the ease of oligoribonucleotide purification and analysis have been significantly enhanced using anion exchange chromatography. These new methods improve the yield and quality of the oligoribonucleotides synthesized. Hammerhead ribozymes synthesized utilizing the described methods exhibited no diminution in catalytic activity.

Published

1995

6. [Untitled]

Author

Foster Todd P, Takahiro Uchida, Richard C. Wardley, Stephen Martin, and Susan Grimm

Subjects

Pharmacology, biology, business.industry, medicine.medical_treatment, Organic Chemistry, Pharmaceutical Science, Dosage form, PLGA, chemistry.chemical_compound, Ovalbumin, chemistry, Antigen, In vivo, Oral administration, Immunology, medicine, biology.protein, Molecular Medicine, Pharmacology (medical), business, Adjuvant, Saline, Biotechnology

Abstract

Poly(lactide-co-glycolide) microspheres containing different loads of OVA (0.05, 0.1, 0.5 and 1.0% w/w) were manufactured by a w/o/w emulsion/solvent evaporation method. Low load efficiencies of less than 20% were observed. Normal size distributions with mean volume diameters ranging from 3.7 to 4.7 microns were obtained for different batches. The in vitro release of OVA from different loaded microspheres showed an expected burst release with all batches. The in vivo dose study (1, 10, 25, 50 micrograms of OVA) was performed by subcutaneous and oral inoculation in mice by single (0 week) or double (0 and 3 weeks) administration of PLGA 50/50 microspheres containing 0.1% OVA. Subcutaneous administration showed an immune response (serum Ig levels by ELISA) statistically (Fisher's paired t-test; P < 0.05) above OVA saline negative controls at 3, 6 and 12 weeks after administration. Oral administration of microspheres produced statistically higher systemic immune responses at the higher doses. Single and double inoculation orally and subcutaneously produced similar serum antibody levels. The in vivo load study was performed by subcutaneous and oral administration to mice of 25 micrograms OVA contained in various loaded (0.05, 0.1, 0.5 and 1.0% w/w) microspheres. Serum immune responses at 3, 6, and 12 weeks after inoculation were statistically above OVA saline controls and were inversely proportional to the OVA load using either route. This observation suggested a relationship between the number of microspheres delivered and the in vivo serum response. Single subcutaneous administration of 0.05 or 0.1% OVA loaded PLGA 50/50 microspheres induced larger immune responses compared with complete Freund's adjuvant.

Published

1994

7. Use of Cationic Lipids to Enhance the Biological Activity of Antisense Oligonucleotides

Author

Susan Grimm, C. Frank Bennett, Hedy Chan, and Ming-Yi Chiang

Subjects

chemistry.chemical_compound, Liposome, Phosphorothioate Oligonucleotides, chemistry, Biochemistry, Base pair, Oligonucleotide, Nucleolus, Cationic polymerization, Pharmaceutical Science, Biological activity, Fluorescein, Biology

Abstract

Antisense oligonucleotides bind to specific mRNA or pre-mRNA sequences through Watson-Crick base pairing, resulting in decreased expression of the targeted protein. The use of cationic lipids to enhance cellular uptake of antisense oligonucleotides is reviewed herein. Cationic lipids such as N[1-(2,3-dioleyloxy)propyl]-N, N, N-trimethylammonium chloride (DOTMA) were found to enhance the biological activity of phosphorothioate oligonucleotides by at least 1000-fold in cell culture. Cationic lipid preparations enhanced both the rate and amount of oligonucleotide which associated with cells. In addition, DOTMA markedly changed the subcellular distribution of the oligonucleotide. In the absence of lipid, fluorescein labelled phosphorothioate oligonucleotides accumulated in discrete cytoplasmic structures. In the presence of cationic lipids, the oligonucleotides concentrated within the nucleus, were excluded from nucleoli, and localized in punctate cytoplasmic structures. The accumulation of the oligon...

Published

1993

8. Two forms of DNA polymerase delta from mouse cells. Purification and properties

Author

S M Herrmann, Mehran Goulian, J W Sackett, and Susan Grimm

Subjects

DNA clamp, biology, DNA polymerase, DNA polymerase II, Cell Biology, Biochemistry, DNA polymerase delta, Molecular biology, Proliferating cell nuclear antigen, biology.protein, Primase, Molecular Biology, DNA polymerase mu, Polymerase

Abstract

A procedure is described for the purification from cultured mouse cells of two DNA polymerase "delta-like" enzymes, as defined by intrinsic 3'-exonuclease activity, inhibition by aphidicolin, and relative insensitivity to N2-(p-n-butylphenyl)-dGTP. One of the two enzymes has been purified to near homogeneity and, similar to the DNA polymerase delta from calf thymus described by Lee et al. (Lee, M. Y. W. T., Tan, C. K., Downey, K. M., and So, A. G. (1984) Biochemistry 23, 1906-1913), it has a total molecular mass of 178 kDa (from sedimentation velocity of 8.0 S and Stokes radius of 54 A) and is composed of one each of 125- and 50-kDa polypeptides. It also resembles the DNA polymerase delta of Lee et al. in being stimulated by proliferating cell nuclear antigen (PCNA). It is the first clear structural and functional counterpart of the calf thymus enzyme. The major difference between the mouse DNA polymerase delta and the calf thymus enzyme of Lee et al. is that, under specific conditions, the mouse enzyme is active with poly(dA).oligo(dT) in the absence of PCNA, whereas the activity of the calf thymus enzyme with this template is reported to be completely dependent on PCNA. The reason for this difference is not known at this time. The second mouse cell enzyme has a molecular mass of 112 kDa (from sedimentation velocity of 6.3 S and Stokes radius of 43.0 A) and consists of a single polypeptide of 123-125 kDa in denaturing gels (p125). On the basis of its apparent formation by dissociation of DNA polymerase delta, and multiple similarities with DNA polymerase delta in enzymatic properties, the p125 is provisionally identified as the 125-kDa polypeptide of DNA polymerase delta. The p125 does not respond to PCNA, suggesting that the 50-kDa polypeptide is required for the stimulation of DNA polymerase delta by PCNA. The presence of the p125 in cell extracts would explain reports that DNA polymerase delta consists of a single polypeptide of approximately 125 kDa and/or thast it has a smaller molecular mass than DNA polymerase delta of Lee et al. and is not affected by PCNA (this does not apply to PCNA-independent DNA polymerase delta-like enzymes with higher molecular mass than the polymerase delta of Lee et al., which have recently been named DNA polymerases epsilon).

Published

1990

9. Purification and properties of an accessory protein for DNA polymerase alpha/primase

Author

Cheryl J. Heard, Susan Grimm, and Mehran Goulian

Subjects

DNA clamp, biology, DNA polymerase, DNA polymerase II, DNA replication, Cell Biology, Biochemistry, DNA polymerase delta, Molecular biology, biology.protein, Primase, Primer (molecular biology), Molecular Biology, Polymerase

Abstract

A protein that stimulates DNA polymerase alpha/primase many-fold on unprimed poly(dT) was purified to homogeneity from extracts of cultured mouse cells. The protein contains polypeptides of approximately 132 and 44 kDa, and the total molecular mass of 150 kDa calculated from Stokes radius (54 A) and sedimentation coefficient (6.7 S) indicates that it contains one each of the two subunits. The purified "alpha accessory factor" (AAF) also stimulates DNA polymerase alpha/primase in the self-primed reaction with unprimed single-stranded DNA. In addition to these effects on the coordinate activities of DNA polymerase alpha and DNA primase, stimulatory effects were also demonstrated separately on both the polymerase and primase activities of the enzyme complex. However, there was no stimulation with DNase-treated ("activated") DNA under normal conditions for assay of DNA polymerase alpha. The stimulatory activity of mouse AAF is highly specific for DNA polymerase alpha/primase; no effect was observed with mouse DNA polymerases beta, gamma, or delta, nor with retroviral, bacteriophage, or bacterial DNA polymerases. Mouse AAF stimulated human DNA polymerase alpha/primase with several different templates, similar to results with the mouse enzyme. However, it had very little effect on the DNA polymerase/primase from either Drosophila embryo or from yeast.

Published

1990

10. Pharmacokinetics of an antiangiogenic ribozyme (ANGIOZYME) in the mouse

Author

Mark A. Reynolds, Tom J. Parry, Susan Grimm, Francine E. Wincott, Jennifer A. Sandberg, Arun B. Agrawal, Karyn Bouhana, Anna M. Gallegos, and Pamela Pavco

Subjects

Angiozyme, medicine.medical_specialty, Angiogenesis, medicine.medical_treatment, Pharmacology, Biology, chemistry.chemical_compound, Mice, Bolus (medicine), Pharmacokinetics, Internal medicine, Genetics, medicine, Animals, RNA, Catalytic, Receptors, Growth Factor, Tissue Distribution, RNA, Messenger, Volume of distribution, Kidney, Neovascularization, Pathologic, Growth factor, Receptor Protein-Tyrosine Kinases, Vascular endothelial growth factor, Mice, Inbred C57BL, medicine.anatomical_structure, Endocrinology, Receptors, Vascular Endothelial Growth Factor, chemistry, Female, Half-Life

Abstract

Vascular endothelial growth factor (VEGF) is a growth factor that contributes to the angiogenesis of developing tumors. To interfere with the action of VEGF, a nuclease-stabilized ribozyme, ANGIOZYME, has been developed against VEGF receptor subtype Flt-1 mRNA. To determine which routes of administration would be useful for systemic delivery of this ribozyme, a dose of 30 mg/kg [32P]ANGIOZYME was administered as an i.v., i.p., or s.c. bolus. Concentrations of ANGIOZYME in plasma, femur, kidney, liver, and lung were examined. ANGIOZYME was well absorbed after i.p. (90%) or s.c. administration (77%), with peak plasma concentrations occurring 30 minutes after dosing. Total body clearance after a single dose of 30 mg/kg ANGIOZYME was 20 ml/min/kg, and the elimination half-life was 33 minutes. The apparent volume of distribution at steady-state ranged from 0.5 to 1.3 L/kg. ANGIOZYME was detected in the four tissues examined through the 3 hour sampling period after i.v. or i.p. administration. After s.c. administration, ANGIOZYME was detected in femur, kidney, and lung but not in the liver. The highest concentrations of ANGIOZYME were found in kidney and femur with all three routes. Because of the rapid and extensive absorption after extravascular injections, either i.p. or s.c. administration could be considered for use in pharmacodynamic studies examining the effects of ANGIOZYME or other ribozymes with similar chemical modifications.

Published

1999

11. Three cytoplasmic DNA polymerases that utilize poly(rA).oligo(dT)

Author

Mehran Goulian and Susan Grimm

Subjects

Cytoplasm, DNA clamp, biology, DNA polymerase, DNA polymerase II, Biophysics, Cell Biology, DNA-Directed DNA Polymerase, Biochemistry, Molecular biology, Chromatography, DEAE-Cellulose, Proliferating cell nuclear antigen, Mice, Oligodeoxyribonucleotides, biology.protein, Tumor Cells, Cultured, Animals, Primase, Primer (molecular biology), Leukemia L1210, Poly A, Molecular Biology, DNA polymerase mu, Polymerase

Abstract

Three DNA polymerases that use poly(rA).oligo(dT) were partially purified from cytoplasmic extracts of cultured mouse cells (after removal of mitochondria), and characterized. One is similar to, and may be the same as, the mitochondrial DNA polymerase gamma. The other two enzymes, one 7.5 S and the other 3.6 S, share some properties with DNA polymerases beta and gamma, e.g. their responses to certain inhibitors; however, they are not clearly identified with any previously well-characterized mammalian DNA polymerases. It is also demonstrated that the response of DNA polymerase gamma to N-ethylmaleimide is template dependent, and that DNA polymerase alpha has an authentic (albeit small) activity with poly(rA).oligo(dT).

Published

1990