Comparison of protocols for removal of melanin from genomic DNA to optimize PCR amplification of DNA purified from highly pigmented lesions

Bianchini, Raquel Alves; Laus, Ana Carolina; Macedo, Graziela; Reis, R. M.; Vazquez, Vinicius de Lima; Vicente, Anna Luiza Silva Almeida

Comparison of protocols for removal of melanin from genomic DNA to optimize PCR amplification of DNA purified from highly pigmented lesions

Authors: Raquel Alves Bianchini
Ana Carolina Laus
Graziela Macedo
R. M. Reis
Vinicius de Lima Vazquez
Anna Luiza Silva Almeida Vicente
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Publisher: Universidade Federal de Santa Catarina (UFSC)
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Abstract

Melanin is produced by melanocytes and protects against DNA damage by ultraviolet light. Unfortunately, the melanin protein present in melanoma tumor cells is often co-purified during DNA extraction, and this contamination may inhibit subsequent PCR methods, which directly impacts research applications and the molecular diagnostic tests needed for targeted therapeutics. There are presently no described purification protocols that efficiently remove melanin from genomic DNA. In this study, we compare six different methods for melanin removal from genomic DNA: Agarose Gel Electrophoresis, 1mg Chelex®-100, Chelex®-100 5%, centrifugation, OneStep™ PCR Inhibitor Removal Kit and centrifugation plus OneStep™ PCR Inhibitor Removal Kit. Each comparison was made using 16 formalin-fixed paraffin-embedded (FFPE) and 11 fresh cell line samples. All samples were initially tested using the multiplex PCR reaction for GAPDH gene that generates different sized amplified products: 100, 200, 300 and 400 base pairs, which could be inhibited by the addition of exogenous melanin. Six purification protocols were then applied, and all samples that amplified at least one GAPDH fragment were sequenced to analyze the presence of the BRAF V600E mutation. The efficiencies of amplification decreased for larger sized fragments in all methods. Our comparisons showed that centrifugation combined with the OneStep™ PCR Inhibitor Removal Kit was superior to all other methods for successful BRAF sequencing with 100% (100bp), 75% (200bp), 50% (300bp), and 31.3% (400bp) amplification efficiencies for the different amplicon sizes. In conclusion, this genomic DNA extraction method is highly efficient for successful PCR when tumor samples are contaminated with melanin.The authors would like to express their sincere thanks to the Sao Paulo Research Foundation (FAPESP) for its funding of this research (Vazquez's Grant #2012/04194-1, Vicente's Doctoral Fellowship Grant #2016/15941-3 and Vicente's International Research Fellowship Grant #2017/09612-0). The authors would like to thank Dr. Jeremy Squire for checking the English and for his critical review of this manuscript

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