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43 results on '"Pyle, A M"'

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1. RNA binding activates RIG-I by releasing an autorepressed signaling domain.

2. Transcriptome analysis of human cumulus cells reveals hypoxia as the main determinant of follicular senescence.

3. Control of branch-site choice by a group II intron.

4. Visualizing the solvent-inaccessible core of a group II intron ribozyme.

5. Guiding ribozyme cleavage through motif recognition: the mechanism of cleavage site selection by a group ii intron ribozyme.

6. Active disruption of an RNA-protein interaction by a DExH/D RNA helicase.

7. Kinetic dissection of the multistep process in L1.ltrB intron mobility.

8. Metal ion binding sites in a group II intron core.

9. A tertiary interaction that links active-site domains to the 5' splice site of a group II intron.

10. New tricks from an itinerant intron.

11. The DExH protein NPH-II is a processive and directional motor for unwinding RNA.

13. Calculating the electrostatic properties of RNA provides new insights into molecular interactions and function.

14. Antagonistic substrate binding by a group II intron ribozyme.

15. Site-specific labeling of RNA with fluorophores and other structural probes.

16. Stepping through an RNA structure: A novel approach to conformational analysis.

17. Defining functional groups, core structural features and inter-domain tertiary contacts essential for group II intron self-splicing: a NAIM analysis.

18. A map of the binding site for catalytic domain 5 in the core of a group II intron ribozyme.

19. More than one way to splice an RNA: branching without a bulge and splicing without branching in group II introns.

20. The architectural organization and mechanistic function of group II intron structural elements.

21. The DEAH-box protein PRP22 is an ATPase that mediates ATP-dependent mRNA release from the spliceosome and unwinds RNA duplexes.

22. Sequence specificity of a group II intron ribozyme: multiple mechanisms for promoting unusually high discrimination against mismatched targets.

23. Group II intron splicing in vivo by first-step hydrolysis.

24. Ribozyme catalysis from the major groove of group II intron domain 5.

25. Stopped-flow fluorescence spectroscopy of a group II intron ribozyme reveals that domain 1 is an independent folding unit with a requirement for specific Mg2+ ions in the tertiary structure.

26. Branch-site selection in a group II intron mediated by active recognition of the adenine amino group and steric exclusion of non-adenine functionalities.

27. Remarkable morphological variability of a common RNA folding motif: the GNRA tetraloop-receptor interaction.

29. Catalytic role of 2'-hydroxyl groups within a group II intron active site.

30. Two competing pathways for self-splicing by group II introns: a quantitative analysis of in vitro reaction rates and products.

31. Role of metal ions in ribozymes.

32. Group II intron ribozymes that cleave DNA and RNA linkages with similar efficiency, and lack contacts with substrate 2'-hydroxyl groups.

33. RNA folding.

34. Branch-point attack in group II introns is a highly reversible transesterification, providing a potential proofreading mechanism for 5'-splice site selection.

35. Conversion of a group II intron into a new multiple-turnover ribozyme that selectively cleaves oligonucleotides: elucidation of reaction mechanism and structure/function relationships.

36. Replacement of the conserved G.U with a G-C pair at the cleavage site of the Tetrahymena ribozyme decreases binding, reactivity, and fidelity.

37. Building a kinetic framework for group II intron ribozyme activity: quantitation of interdomain binding and reaction rate.

38. Ribozymes: a distinct class of metalloenzymes.

40. RNA substrate binding site in the catalytic core of the Tetrahymena ribozyme.

41. Ribozyme recognition of RNA by tertiary interactions with specific ribose 2'-OH groups.

42. Direct measurement of oligonucleotide substrate binding to wild-type and mutant ribozymes from Tetrahymena.

43. High resolution footprinting of EcoRI and distamycin with Rh(phi)2(bpy)3+, a new photofootprinting reagent.

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