dna stabilization
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eLife ◽  
2020 ◽  
Vol 9 ◽  
Author(s):  
Jose F Moruno-Manchon ◽  
Pauline Lejault ◽  
Yaoxuan Wang ◽  
Brenna McCauley ◽  
Pedram Honarpisheh ◽  
...  

Guanine-rich DNA sequences can fold into four-stranded G-quadruplex (G4-DNA) structures. G4-DNA regulates replication and transcription, at least in cancer cells. Here, we demonstrate that, in neurons, pharmacologically stabilizing G4-DNA with G4 ligands strongly downregulates the Atg7 gene. Atg7 is a critical gene for the initiation of autophagy that exhibits decreased transcription with aging. Using an in vitro assay, we show that a putative G-quadruplex-forming sequence (PQFS) in the first intron of the Atg7 gene folds into a G4. An antibody specific to G4-DNA and the G4-DNA-binding protein PC4 bind to the Atg7 PQFS. Mice treated with a G4 stabilizer develop memory deficits. Brain samples from aged mice contain G4-DNA structures that are absent in brain samples from young mice. Overexpressing the G4-DNA helicase Pif1 in neurons exposed to the G4 stabilizer improves phenotypes associated with G4-DNA stabilization. Our findings indicate that G4-DNA is a novel pathway for regulating autophagy in neurons.


Molecules ◽  
2019 ◽  
Vol 24 (8) ◽  
pp. 1473 ◽  
Author(s):  
Dora M. Răsădean ◽  
Samuel W. O. Harrison ◽  
Isobel R. Owens ◽  
Aucéanne Miramont ◽  
Frances M. Bromley ◽  
...  

Four pairs of amino acid-functionalized naphthalenediimide enantiomers (d- and l-lysine derived NDIs) were screened toward G-quadruplex forming sequences in telomeres (h-TELO) and oncogene promoters: c-KIT1, c-KIT2, k-RAS and BCL-2. This is the first study to address the effect of point chirality toward G-quadruplex DNA stabilization using purely small organic molecules. Enantioselective behavior toward the majority of ligands was observed, particularly in the case of parallel conformations of c-KIT2 and k-RAS. Additionally, Nε-Boc-l-Lys-NDI and Nε-Boc-d-Lys-NDI discriminate between quadruplexes with parallel and hybrid topologies, which has not previously been observed with enantiomeric ligands.


2017 ◽  
Author(s):  
Riley Hughes ◽  
Zeynep Alkan ◽  
Nancy L. Keim ◽  
Mary E. Kable

ABSTRACTBackgroundThe human gut microbiome has been widely studied in the context of human health and metabolism, however the question of how to analyze this community remains contentious. This study compares new and previously well established methods aimed at reducing bias in bioinformatics analysis (QIIME 1 and DADA2) and bacterial DNA extraction of human fecal samples in 16S rRNA marker gene surveys.ResultsAnalysis of a mock DNA community using DADA2 identified more chimeras (QIIME 1: 0.70% of total reads vs DADA2: 1.96%), fewer sequence variants, (QIIME 1: 1297.4 + 98.88 vs. DADA2: 136.27 + 11.35, mean + SD) and correct taxa at a higher resolution of classification (i.e. genus-level) than open reference OTU picking in QIIME 1. Additionally, the extraction of whole cell mock community bacterial DNA using four commercially available kits resulted in varying DNA yield, quality and bacterial community composition. Of the four kits compared, ZymoBIOMICS DNA Miniprep Kit provided the greatest yield, with a slight enrichment of Enterococcus. However, QIAamp Fast DNA Stool Mini Kit resulted in the highest DNA quality. Mo Bio PowerFecal DNA Kit had the most dramatic effect on the mock community composition, resulting in an increased proportion of members of the family Enterobacteriaceae and genus Eshcerichia as well as members of genera Lactobacillus and Pseudomonas. The presence of a sterile fecal matrix had a slight, but inconsistent effect on the yield, quality and taxa identified after extraction with all four DNA extraction kits. Extraction of bacterial DNA from native stool samples revealed a distinct effect of the DNA stabilization reagent DNA/RNA Shield on community composition, causing an increase in the detected abundance of members of orders Bifidobacteriales, Bacteroidales, Turicibacterales, Clostridiales and Enterobacteriales.ConclusionThese results confirm that the DADA2 algorithm is superior to sequence clustering by similarity to determine microbial community structure. Additionally, commercially available kits used for bacterial DNA extraction from fecal samples have some effect on the proportion of high abundance members detected in a microbial community, but it is less significant than the effect of using DNA stabilization reagent, DNA/RNA Shield.


Biochemistry ◽  
2017 ◽  
Vol 56 (33) ◽  
pp. 4392-4404 ◽  
Author(s):  
Kranthikumar Yadav ◽  
Penchala Narasimha Rao Meka ◽  
Sudeshna Sadhu ◽  
Sravanthi Devi Guggilapu ◽  
Jeshma Kovvuri ◽  
...  

2015 ◽  
Vol 13 (34) ◽  
pp. 8996-8999 ◽  
Author(s):  
Jiaqi Wang ◽  
Shaoru Wang ◽  
Cheng Zhong ◽  
Tian Tian ◽  
Xiang Zhou

Here, we have provided novel insights into the effects of 8-oxodG substitutions on B–Z transitions of CpG dinucleotide DNAs.


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