Comparison of multiple genotyping methods for the identification of the cancer predisposing founder mutation p.R337H in <i>TP53</i>

Fitarelli-Kiehl, Mariana; Macedo, Gabriel S.; Schlatter, Rosane Paixão; Koehler-Santos, Patricia; Matte, Ursula da Silveira; Ashton-Prolla, Patricia; Giacomazzi, Juliana

doi:10.1590/1678-4685-GMB-2014-0351

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Genetics and Molecular Biology

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Special Oncogenetics • Genet. Mol. Biol. 39 (2) • Apr-Jun 2016 • https://doi.org/10.1590/1678-4685-GMB-2014-0351 copy

Comparison of multiple genotyping methods for the identification of the cancer predisposing founder mutation p.R337H in TP53

Authorship SCIMAGO INSTITUTIONS RANKINGS

Abstract

Germline mutations in the TP53 gene are associated with Li-Fraumeni and Li-Fraumeni-Like Syndromes, characterized by increased predisposition to early-onset cancers. In Brazil, the prevalence of the TP53-p.R337H germline mutation is exceedingly high in the general population and in cancer-affected patients, probably as result of a founder effect. Several genotyping methods are used for the molecular diagnosis of LFS/LFL, however Sanger sequencing is still considered the gold standard. We compared performance, cost and turnaround time of Sanger sequencing, PCR-RFLP, TaqMan-PCR and HRM in the p.R337H genotyping. The performance was determined by analysis of 95 genomic DNA samples and results were 100% concordant for all methods. Sequencing was the most expensive method followed by TaqMan-PCR, PCR-RFLP and HRM. The overall cost of HRM increased with the prevalence of positive samples, since confirmatory sequencing must be performed when a sample shows an abnormal melting profile, but remained lower than all other methods when the mutation prevalence was less than 2.5%. Sequencing had the highest throughput and the longest turnaround time, while TaqMan-PCR showed the lowest turnaround and hands-on times. All methodologies studied are suitable for the detection of p.R337H and the choice will depend on the application and clinical scenario.

Keywords
TP53-p.R337H; RFLP; TaqMan; HRM; Sanger Sequencing

	Sanger Sequencing^a a 96-well plates	PCR-RFLP^b b 2 × 31-well gels	TaqMan-PCR^c c 48-well plates.	HRM^c c 48-well plates.
Negative controls (GG genotype)	0	1	1	3
Positive controls (GA or AA genotypes)	0	2	2	2
Patient samples tested per run^d d bidirectional sequencing, duplicate analyses for all other methods	47	27	22	21
Throughput (full capacity)	96	62	48	48
Total turnaround time (hours)^e e does not include DNA isolation and quantification.	37	13.5	3	5.25
Hands-on time (hours)	13.5	3	1	1.25

Description	HRM^c c HRM is a screening method and not a direct genotyping method as PCR-RFLP, TaqMan and Sanger sequencing (see Figure 2 for further details on additional cost).	PCR-RFLP	TaqMan-PCR	DNA Sequencing
Total cost (R$)^a a includes DNA isolation, quantification, all steps of each method and professional labor cost for handling and result interpretation	18.84	19.86	26.28	53.29
Fold increase of cost^b b in relation to the least expensive method	1.00	1.05	1.39	2.83

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[1] Send correspondence to Patricia Ashton-Prolla. Laboratório de Medicina Genômica, Centro de Pesquisa Experimental, Hospital de Clínicas de Porto Alegre, Rua Ramiro Barcelos, 2350, 90035-903 Porto Alegre, RS, Brazil. E-mail: pprolla@hcpa.edu.br.