Manipulation of primer affinity improves high-resolution melting accuracy for imprinted genes

Fv, Rubatino; Carobin, Natália Virtude; Ml, Freitas; Vt, de Oliveira; Rx, Pietra; Pp, Oliveira; Aa, Bosco; Fs, Jehee

doi:10.4238/2015.july.14.12

Cited by 4 publications

(3 citation statements)

References 14 publications

(30 reference statements)

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“…However, several important points about the HRM method have been proposed; improved efficiency is probably due to the short length of primers, which enabled better amplification in PCR. Furthermore, the concentration of primers has an important role in increasing the sensitivity and specificity of HRM assay (Rubatino et al ; Słomka et al ). The sensitivity of these primers performed that with this technology, template DNA can be amplified exponentially starting from very low concentrations in the initial sample.…”

Section: Resultsmentioning

confidence: 99%

New approach to identify colistin‐resistant Pseudomonas aeruginosa by high‐resolution melting curve analysis assay

Tahmasebi

Dehbashi

Arabestani

2020

Lett Appl Microbiol

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Colistin‐resistant Pseudomonas aeruginosa (CRPA), as a health care system threat, is increasing globally. This study aimed was to determine CRPA by high‐resolution melting curve (HRM) analysis method. The HRM method was done on standard strains of P. aeruginosa and CRPA strains. Ninefold serial dilutions of known genomic DNA (gDNA) and plasmid DNA (pDNA) concentrations, extracted from P. aeruginosa NCTC13715 and P. aeruginosa NCTC10728 were prepared and tested by melting curve analysis and HRM assay. Data analysis was performed using the Step‐One Plus Software v2.3 and hrm Software v3.0.1. The results of the melt curve analysis and HRM showed a very similar melt peak for all positive controls with a melt temperature that ranged from 88·1°C to 88·6°C for the 16srRNA, 90·0°C to 90·05°C for the mcr‐1 and 91·2°C to 91·7°C for the pmrA gene. Furthermore, the data indicated that the HRM approach has the sensitivity to detect 100 CFU per ml for the 16srRNA gene, 101 CFU per ml for the pmrA gene, and 103 CFU per ml for the mcr‐1 gene. According to our findings, it was concluded that the HRM method could detect 100 to 103 CFU per ml of P. aeruginosa gDNA and pDNA. Therefore, CRPA strains can be identified with high sensitivity and specificity by HRM assay. Significance and Impact of the Study The highlight of our research is about the detection of bacteria resistance genes to antibiotics by advanced molecular methods, which means high‐resolution melting curve (HRM) analysis. We determined that the HRM method in identifying colistin‐resistant P. aeruginosa has high accuracy and speed, and with high sensitivity and specificity.

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Section: Resultsmentioning

confidence: 99%

New approach to identify colistin‐resistant Pseudomonas aeruginosa by high‐resolution melting curve analysis assay

Tahmasebi

Dehbashi

Arabestani

2020

Lett Appl Microbiol

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“…Although aforementioned results were consistent with PWS, genetic testing was resumed at 12 years of age due to their atypical phenotype. Methylation‐sensitive high resolution melting (MS‐HRM) (Rubatino et al, ), performed on peripheral blood DNA, confirmed methylation of the SNURF‐SNRPN promoter in both twins (Supplementary Figure S2). Taking into consideration the presence of some symptoms of Angelman Syndrome (AS, MIM #105830) such as apparent ID, microcephaly, lack of speech, autistic features, and epilepsy, it was hypothesized that the UBE3A gene on the non‐deleted chromosome was potentially silenced by a mutation.…”

Section: Clinical Reportmentioning

confidence: 65%

Dual molecular diagnosis contributes to atypical Prader–Willi phenotype in monozygotic twins

Jehee

Oliveira

Gurgel-Giannetti

et al. 2017

American J of Med Genetics Pt A

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We describe monozygotic twin girls with genetic variation at two separate loci resulting in a blended phenotype of Prader-Willi syndrome and Pitt-Hopkins syndrome. These girls were diagnosed in early infancy with Prader-Willi syndrome, but developed an atypical phenotype, with apparent intellectual deficiency and lack of obesity. Array-comparative genomic hybridization confirmed the apparently de novo paternal deletion of the 15q11.2q13 region and exome sequencing identified a second mutational event in both girls, which was a novel variant c.145+1G>A affecting a TCF4 canonical splicing site inherited from the mosaic mother. RNA studies showed that the splice site variant abolished the donor splicing site, which was accompanied by activation of an alternative non-canonical splicing-site which then predicts a premature stop codon in the following exon. Clinical re-evaluation of the twins showed that both variants are likely contributing to the more severe phenotypic presentation. Our data show that atypical clinical presentations may actually be the expression of blended clinical phenotypes arising from independent pathogenic events at two loci.

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“…Primers sequences for the amplification of the SNRPN (NG_012958.1) gene were designed based on the methodologies of Rubatino et al, 2015. In summary, the designed forward primer established a perfect match with the unmethylated template, while the reverse primer exhibited one mismatch with the methylated template.…”

Section: Primer Design and Sequencesmentioning

confidence: 99%

Methylation profile of SNRPN gene and its correlation with weight and chronological age

et al. 2015

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ABSTRACT. Genomic imprinting is an important epigenetic phenomenon, wherein genes or gene clusters are marked by DNA methylation during gametogenesis. This plays a major role in several functions of normal cells, including cell differentiation, X chromosome inactivation, and the maintenance of chromatin structure, in mammalian development. The aim of this study was to investigate the possible differences in SNRPN gene methylation profiles in non-obese and obese individuals, and in children and adults. Our results did not reveal any statistical correlations between the DNA methylation profiles of the SNRPN gene in children or adult obese and non-obese groups. However, a comparison of the methylation levels with the chronological age revealed statistically significant differences between the means of methylation in adults and children (46.20 ± 5.88 and 39.40 ± 2.87, respectively; P < 0.001). Pearson's correlation analysis indicated a positive association between the level of DNA methylation and the chronological age (R 2 = 0.326; P < 0.001). Therefore, we concluded that the methylation profile of the SNRPN promoter (in blood) is not a useful biomarker for determining the predisposition of an individual to obesity. Additionally, we have confirmed that SNRPN methylation increases with 13791-13798 (2015) age, which raises further questions regarding the role of SNRPN expression during the aging process.

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Manipulation of primer affinity improves high-resolution melting accuracy for imprinted genes

Cited by 4 publications

References 14 publications

New approach to identify colistin‐resistant Pseudomonas aeruginosa by high‐resolution melting curve analysis assay

New approach to identify colistin‐resistant Pseudomonas aeruginosa by high‐resolution melting curve analysis assay

Dual molecular diagnosis contributes to atypical Prader–Willi phenotype in monozygotic twins

Methylation profile of SNRPN gene and its correlation with weight and chronological age

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