Protein hnRNP A1 and its derivative Up1 unfold quadruplex DNA in the human KRAS promoter: implications for transcription

Paramasivam, Manikandan; Membrino, Alexandro; Cogoi, Susanna; Fukuda, Hirokazu; Nakagama, Hitoshi; Xodo, Luigi E.

doi:10.1093/nar/gkp138

Cited by 131 publications

(129 citation statements)

References 47 publications

(93 reference statements)

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“…The affinity of MAZ-GST for the parallel hras -2 quadruplex is 2.4-fold higher than for the antiparallel hras -1 quadruplex. The K D 's between MAZ-GST and HRAS quadruplexes are not so different from those reported for the binding of recombinant UP1, hRNP A1, nucleophosmin and nucleolin to G4-DNA (26–28). Instead, the K D reported for the interaction between cellular Sp1 and quadruplex cKIT is >10-fold lower (29).…”

Section: Resultscontrasting

confidence: 66%

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HRASis silenced by two neighboring G-quadruplexes and activated by MAZ, a zinc-finger transcription factor with DNA unfolding property

2014

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The HRAS promoter contains immediately upstream of the transcription start site two neighboring G-elements, each capable of folding into a G-quadruplex structure. We have previously found that these G-quadruplexes bind to the zinc-finger transcription factors MAZ and Sp1. In the present study we have examined the interaction between the HRAS promoter and MAZ, demonstrating for the first time that the protein unfolds the G-quadruplex structures. We also demonstrate that MAZ-GST, in the presence of the complementary strands, promotes a rapid transformation of the two HRAS quadruplexes into duplexes. By a mutational analysis of the HRAS G-elements, we dissected the MAZ-binding sites from the quadruplex-forming motifs, finding that the two neighboring G-quadruplexes bring about a dramatic repression of transcription, in a synergistic manner. We also discovered that the two G-quadruplexes are strong targets for small anticancer molecules. We found that a cell-penetrating anthratiophenedione (ATPD-1), which binds tightly to the G-quadruplexes (ΔT > 15°C), promotes the total extinction of HRAS transcription. In contrast, when one of the two G-quadruplexes was abrogated by point mutations, ATPD-1 repressed transcription by only 50%. Our study provides relevant information for the rationale design of targeted therapy drugs specific for the HRAS oncogene.

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Section: Resultscontrasting

confidence: 66%

“…The unfolding process can be followed by fluorescence-resonance energy transfer (FRET), using hras -1 and hras -2 quadruplex-forming sequences tagged at the 5′ and 3′ ends with FAM (donor) and TAMRA (acceptor) [F- hras 1-T, F- hras 2-T] (26,30,31). In Figure 4A we report the data obtained with the antiparallel hras -1 quadruplex.…”

Section: Resultsmentioning

confidence: 99%

HRASis silenced by two neighboring G-quadruplexes and activated by MAZ, a zinc-finger transcription factor with DNA unfolding property

2014

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“…However, it is possible that specific nuclear proteins could promote and/or stabilize i-motif structures under physiological conditions in vivo (56,(67)(68)(69)(70). The formation of an i-motif structure by a C-rich motif associated with a meiosis-specific DSB at a near-neutral pH supports the notion that this structure is physiologically relevant.…”

Section: Discussionmentioning

confidence: 78%

“…Indeed, a number of proteins have been shown to bind cytosinerich strands, possibly i-motif structures. Examples include hnRNP A1 (67,68), hnRNP K (69,70), hnRNP LL (56), the Trypanosoma brucei ST-1 protein (71), and the rat nuclear protein qTBP42 (72). On the basis of the reports described above, it is apparent that i-motif structures can serve as attractive drug targets for anti-cancer therapy (56,73,74).…”

Section: Introductionmentioning

confidence: 99%

Probing the Potential Role of Non-B DNA Structures at Yeast Meiosis-Specific DNA Double-Strand Breaks

Kshirsagar

Khan

Hosur

et al. 2017

Biophysical Journal

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A plethora of evidence suggests that different types of DNA quadruplexes are widely present in the genome of all organisms. The existence of a growing number of proteins that selectively bind and/or process these structures underscores their biological relevance. Moreover, G-quadruplex DNA has been implicated in the alignment of four sister chromatids by forming parallel guanine quadruplexes during meiosis; however, the underlying mechanism is not well defined. Here we show that a G/C-rich motif associated with a meiosis-specific DNA double-strand break (DSB) in Saccharomyces cerevisiae folds into G-quadruplex, and the C-rich sequence complementary to the G-rich sequence forms an i-motif. The presence of G-quadruplex or i-motif structures upstream of the green fluorescent protein-coding sequence markedly reduces the levels of gfp mRNA expression in S. cerevisiae cells, with a concomitant decrease in green fluorescent protein abundance, and blocks primer extension by DNA polymerase, thereby demonstrating the functional significance of these structures. Surprisingly, although S. cerevisiae Hop1, a component of synaptonemal complex axial/lateral elements, exhibits strong affinity to G-quadruplex DNA, it displays a much weaker affinity for the i-motif structure. However, the Hop1 C-terminal but not the N-terminal domain possesses strong i-motif binding activity, implying that the C-terminal domain has a distinct substrate specificity. Additionally, we found that Hop1 promotes intermolecular pairing between G/C-rich DNA segments associated with a meiosis-specific DSB site. Our results support the idea that the G/C-rich motifs associated with meiosis-specific DSBs fold into intramolecular G-quadruplex and i-motif structures, both in vitro and in vivo, thus revealing an important link between non-B form DNA structures and Hop1 in meiotic chromosome synapsis and recombination.

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“…The identification of G-quadruplex-binding proteins such as nucleolin [15] and NM23-H2 [16] seems to provide strong circumstantial evidence of the existence of G-quadruplexes in living organisms. In addition to the human telomeric G-quadruplexes formed from TTAGGG repeats, bioinformatics analysis has revealed an over-representation of G-quadruplex-forming sequences in the promoter regions of genes, including oncogenes such as c-myc [17][18][19], bcl-2 [20,21], VEGF [22][23][24], KRAS [25,26], c-kit [27][28][29][30][31] and RET [32,33]. Thus, G-quadruplexes have been proposed to be intimately associated with various biological processes such as transcriptional control of gene expression and the regulation of the cell cycle and apoptosis.…”

Section: Introductionmentioning

confidence: 99%

In silico screening of quadruplex-binding ligands

Pui‐Yan

Chan

et al. 2012

Methods

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Protein hnRNP A1 and its derivative Up1 unfold quadruplex DNA in the human KRAS promoter: implications for transcription

Cited by 131 publications

References 47 publications

HRASis silenced by two neighboring G-quadruplexes and activated by MAZ, a zinc-finger transcription factor with DNA unfolding property

HRASis silenced by two neighboring G-quadruplexes and activated by MAZ, a zinc-finger transcription factor with DNA unfolding property

Probing the Potential Role of Non-B DNA Structures at Yeast Meiosis-Specific DNA Double-Strand Breaks

In silico screening of quadruplex-binding ligands

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