Neuronal Expression of Neural Nitric Oxide Synthase (nNOS) Protein Is Suppressed by an Antisense RNA Transcribed from an NOS Pseudogene

Korneev, Sergei A.; Park, Ji-Ho; O’Shea, Michael

doi:10.1523/jneurosci.19-18-07711.1999

Cited by 253 publications

(214 citation statements)

References 31 publications

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“…Transcription of a pseudogene that is homologous to the neuronal nitric oxide synthase (nNOS) gene in a population of neurons decreases the expression levels for the nNOS gene. Interestingly, RNA isolated from these neuronal cells confirmed the presence of an in vivo stable RNA-RNA duplex between these two transcripts suggested to arise via a reversecomplement sequence found at the 5Ј end of the pseudo-NOS transcript (Korneev et al 1999). This study implicated the pseudo-NOS transcript as a natural antisense regulator of nNOS protein synthesis (Korneev et al 1999).…”

Section: Pseudogene Transcripts: No More 'Junk'mentioning

confidence: 68%

“…A role of pseudogene transcripts in gene regulation has also been reported in the snail Lymnea stagnalis (Korneev et al 1999(Korneev et al , 2005. Transcription of a pseudogene that is homologous to the neuronal nitric oxide synthase (nNOS) gene in a population of neurons decreases the expression levels for the nNOS gene.…”

Section: Pseudogene Transcripts: No More 'Junk'mentioning

confidence: 98%

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Eukaryotic regulatory RNAs: an answer to the ‘genome complexity’ conundrum

Prasanth¹,

Spector²

2007

Genes Dev.

364

305

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A large portion of the eukaryotic genome is transcribed as noncoding RNAs (ncRNAs). While once thought of primarily as "junk," recent studies indicate that a large number of these RNAs play central roles in regulating gene expression at multiple levels. The increasing diversity of ncRNAs identified in the eukaryotic genome suggests a critical nexus between the regulatory potential of ncRNAs and the complexity of genome organization. We provide an overview of recent advances in the identification and function of eukaryotic ncRNAs and the roles played by these RNAs in chromatin organization, gene expression, and disease etiology.

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Section: Pseudogene Transcripts: No More 'Junk'mentioning

confidence: 68%

Section: Pseudogene Transcripts: No More 'Junk'mentioning

confidence: 98%

Eukaryotic regulatory RNAs: an answer to the ‘genome complexity’ conundrum

Prasanth¹,

Spector²

2007

Genes Dev.

364

305

View full text Add to dashboard Cite

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“…Although the process of retrotransposition may have been necessary for genome evolution (36), the vast majority of existing pseudogenes are considered as ''junk'' DNA. Although some are transcribed, many have accumulated mutations that would preclude function, and only a very small number may play physiological roles (37)(38)(39). Indeed, even though exon shuffling may have been of great importance in the evolutionary past (40,41), the Trim5-CypA protein appears to belong to a tiny handful of functional proteins unambiguously created in this manner.…”

Section: Discussionmentioning

confidence: 99%

A Trim5-cyclophilin A fusion protein found in owl monkey kidney cells can restrict HIV-1

Nisole¹,

Lynch²,

Stoye³

et al. 2004

Proc. Natl. Acad. Sci. U.S.A.

280

303

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Lv1 restriction of HIV-1 in the cells of Old World monkeys is associated with the expression of the Trim5 gene. Uniquely, in owl monkey kidney cells, HIV-1 restriction is dependent on the ability of incoming viral capsid protein to bind cyclophilin A (CypA). Cloning of the owl monkey Trim5 gene now reveals the presence of an inserted CypA pseudogene within intron 7 of the Trim5 gene. This insertion results in the formation of a chimeric Trim5-CypA transcript. Transfer of a cDNA corresponding to this transcript into human cells confers cyclosporin A-sensitive resistance to HIV-1 infection. The restriction factor appears to be a chimeric protein created by retrotransposon-mediated exon shuffling

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“…PCR ampliWcation of products longer than 4.5 kb were ampliWed with the Expand High Fidelity system (ROCHE), using ampliWcation programs as indicated in the manufacturer's instructions. Doublestranded RNA was detected according to the protocol described in Korneev (1999). The list of the primers used in this study is found in supplementary Materials and methods, Table 1.…”

Section: Genome Walkmentioning

confidence: 99%

“…The smear at the bottom of the Southern blot is likely due to breakdown of the radioactively labelled Wrst strand during PCR and/or linear ampliWcation of breakdown products which have lost one primer-annealing site, but which still can hybridise to the radioactive probe Parts of RSI RNA and the TNP RNA form double-stranded RNA The detection of the RSI-ATs suggested that doublestranded RNAs (dsRNA) might form in cells where both RSI and RSI-ATs transcripts are expressed. To detect dsRNA we took advantage of the methods described in Korneev et al (1999), which exploited the feature of the RNase-ONE enzyme to degrade single-stranded RNA leaving dsRNA intact. Total RNA was extracted under non-denaturing conditions, treated with an excess of RNase-ONE and reverse-transcribed with primers located outside and inside the hypothetical dsRNA molecules (Fig.…”

Section: Fig 3 Detection Of Tamrsi-2 Transposition (A B) and Three mentioning

confidence: 99%

ROSINA (RSI) is part of a CACTA transposable element, TamRSI, and links flower development to transposon activity

Roccaro¹,

Sommer³

et al. 2007

Mol Genet Genomics

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ROSINA (RSI) was isolated as a DNA binding factor able to bind to the CArG-box present in the promoter of the MADS-box gene DEFICIENS of Antirrhinum majus. The mosaic nature of RSI and its multi-copy presence in the A. majus genome indicated that RSI could be a part of a mobile genetic element. Here we show that RSI is a part of a CACTA transposable element system of A. majus, named TamRSI, which has evolved and is still evolving within the terminal inverted repeats (TIRs) of this CACTA transposon. Interestingly, RSI is always found in opposite orientation with respect to the transcription of a second gene present within the CACTA transposon, which encodes a putative TRANSPOSASE (TNP). This structural conWguration has not yet been described for any member of the CACTA transposons superfamily. Internal deletion derivatives of the TamRSI produce aberrant RSI transcripts (RSIATs) that carry parts of the RSI RNA fused to parts of the TNP RNA. In addition, an intriguing seed phenotype shown by RNAi transgenic lines generated to silence RSI, relate TamRSI to epigenetic mechanisms and associate the control of Xower development to transposon activity.

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Neuronal Expression of Neural Nitric Oxide Synthase (nNOS) Protein Is Suppressed by an Antisense RNA Transcribed from an NOS Pseudogene

Cited by 253 publications

References 31 publications

Eukaryotic regulatory RNAs: an answer to the ‘genome complexity’ conundrum

Eukaryotic regulatory RNAs: an answer to the ‘genome complexity’ conundrum

A Trim5-cyclophilin A fusion protein found in owl monkey kidney cells can restrict HIV-1

ROSINA (RSI) is part of a CACTA transposable element, TamRSI, and links flower development to transposon activity

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