2020
DOI: 10.1016/j.jmb.2019.09.002
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Functional Conservation of LncRNA JPX Despite Sequence and Structural Divergence

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Cited by 39 publications
(31 citation statements)
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References 90 publications
(153 reference statements)
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“…Overexpression of human JPX RNA in trans was recently shown to complement heterozygous deletion of mouse Jpx during the establishment of XCI, suggesting that the human RNA might be functional in an ectopic context (Karner et al, 2019). Such rescue experiments using orthologous LRGs, as opposed to our strategy to tackle the role of mouse and human Jpx/JPX in the respective 5 species, reveal the effect of the environment on LRG mode of action but do not interrogate LRGs' function in their endogenous contexts.…”
Section: Xist P510mentioning
confidence: 96%
“…Overexpression of human JPX RNA in trans was recently shown to complement heterozygous deletion of mouse Jpx during the establishment of XCI, suggesting that the human RNA might be functional in an ectopic context (Karner et al, 2019). Such rescue experiments using orthologous LRGs, as opposed to our strategy to tackle the role of mouse and human Jpx/JPX in the respective 5 species, reveal the effect of the environment on LRG mode of action but do not interrogate LRGs' function in their endogenous contexts.…”
Section: Xist P510mentioning
confidence: 96%
“…First, as mentioned above, many lncRNAs have been found only in cell lines and their patterns of expression in vivo are not known. Second, due to low sequence conservation of mammalian lncRNAs [138], the homologs of human transcripts in animal models may be unknown due to deep divergence in sequence and structure [216] or may not even exist. Third, human lncRNAs found only in cell lines can still have properties making them attractive for in-depth analysis, for example involvement in drug resistance, leaving the cell lines as the only logical choice for these assays.…”
Section: Emerging Solutions To Address the Challenge Of Uncovering Trmentioning
confidence: 99%
“…Plasmid preparation and transfection were carried out as previously described [9]. Hela cells were cultured in minimum essential medium (MEM; Thermo fisher, USA), supplemented with 10% fetal bovine serum, and incubated under 5% CO 2 at 37 °C.…”
Section: Plasmid Construction and Transfectionmentioning
confidence: 99%
“…RNA extraction and quantitative real-time PCR (qRT-PCR) were carried out as previously described [9]. Total RNAs were extracted using Trizol reagent (Invitrogen, Carlsbad, CA).…”
Section: Rna Extraction and Quantitative Real-time Pcr (Qrt-pcr)mentioning
confidence: 99%