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Pivot Concepts:
Gene/Protein
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Target Concepts:
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Query: EC:2.7.7.48 (
transcriptase
)
9,479
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Post-transcriptional gene silencing (PTGS) involving small interfering RNA (siRNA)-directed degradation of RNA transcripts and transcriptional silencing via DNA methylation have each been proposed as mechanisms of genome defence against invading nucleic acids, such as transposons and viruses. Furthermore, recent data from plants indicates that many transposons are silenced via a combination of the two mechanisms, and siRNAs can direct methylation of transposon sequences. We investigated the contribution of DNA methylation and the PTGS pathway to transposon control in the filamentous fungus Neurospora crassa. We found that repression of the LINE1-like transposon, Tad, requires the Argonaute protein QDE2 and Dicer, each of which are required for transgene-induced PTGS (quelling) in N.crassa. Interestingly, unlike quelling, the
RNA-dependent RNA polymerase
QDE1 and the RecQ DNA helicase QDE3 were not required for Tad control, suggesting the existence of specialized silencing pathways for diverse kinds of repetitive elements. In contrast, Tad elements were not significantly methylated and the
DIM2
DNA methyltransferase, responsible for all known DNA methylation in Neurospora, had no effect on Tad control. Thus, an RNAi-related transposon silencing mechanism operates during the vegetative phase of N.crassa that is independent of DNA methylation, highlighting a major difference between this organism and other methylation-proficient species.
...
PMID:The post-transcriptional gene silencing machinery functions independently of DNA methylation to repress a LINE1-like retrotransposon in Neurospora crassa. 1576 81
The effort to understand the molecular biology of rotaviruses (RVs) has led to the development of procedures that can be used to study the replication and transcription of the RV genome, the assembly and structure of the rotavirion, and the structure and function of RV proteins. Because it is not possible to provide a detailed description of all the techniques developed, this chapter stresses only those that have broad application, or which represent important new technical advances. In particular, this chapter emphasizes procedures used to prepare large amounts of purified triple-(TLP), double-(
DLP
), and single-layered (core) RV particles; to synthesize viral RNAs in vitro, through the
transcriptase
and replicase activities associated with RV particles; to evaluate the RNA-binding activity of RV proteins; and to assemble core-like and virus-like particles (CLPs and VLPs, respectively) via the expression of RV recombinant proteins.
...
PMID:Virus replication. 2131 54
Rotaviruses, like other non-enveloped, double-strand RNA viruses, package an
RNA-dependent RNA polymerase
(RdRp) with each duplex of their segmented genomes. Rotavirus cell entry results in loss of an outer protein layer and delivery into the cytosol of an intact, inner capsid particle (the "double-layer particle," or
DLP
). The RdRp, designated VP1, is active inside the
DLP
; each VP1 achieves many rounds of mRNA transcription from its associated genome segment. Previous work has shown that one VP1 molecule lies close to each 5-fold axis of the icosahedrally symmetric
DLP
, just beneath the inner surface of its protein shell, embedded in tightly packed RNA. We have determined a high-resolution structure for the rotavirus VP1 RdRp in situ, by local reconstruction of density around individual 5-fold positions. We have analyzed intact virions ("triple-layer particles"), non-transcribing DLPs and transcribing DLPs. Outer layer dissociation enables the
DLP
to synthesize RNA, in vitro as well as in vivo, but appears not to induce any detectable structural change in the RdRp. Addition of NTPs, Mg
2+
, and S-adenosylmethionine, which allows active transcription, results in conformational rearrangements, in both VP1 and the
DLP
capsid shell protein, that allow a transcript to exit the polymerase and the particle. The position of VP1 (among the five symmetrically related alternatives) at one vertex does not correlate with its position at other vertices. This stochastic distribution of site occupancies limits long-range order in the 11-segment, double-strand RNA genome.
...
PMID:In situ Structure of Rotavirus VP1 RNA-Dependent RNA Polymerase. 3123 64
