Comparison of six methods for Loa loa genomic DNA extraction

Roland Dieki; Elsa-Rush Eyang-Assengone; Patrice Makouloutou-Nzassi; Félicien Bangueboussa; Edouard Nsi Emvo; Jean Paul Akue

doi:10.1371/journal.pone.0265582

Comparison of six methods for Loa loa genomic DNA extraction

PLoS One. 2022 Mar 21;17(3):e0265582. doi: 10.1371/journal.pone.0265582. eCollection 2022.

Authors

Roland Dieki^{1

2}, Elsa-Rush Eyang-Assengone³, Patrice Makouloutou-Nzassi³, Félicien Bangueboussa³, Edouard Nsi Emvo², Jean Paul Akue¹

Affiliations

¹ Département de Parasitologie, Centre International de Recherches Médicales de Franceville (CIRMF), Franceville, Gabon.
² Laboratoire de Recherche en Biochimie (LAREBIO), Faculté des Sciences, Université des Sciences et Techniques de Masuku (USTM), Franceville, Gabon.
³ Unité de Recherches en Ecologie de la Santé (URES/CIRMF), BP. 769 Franceville, Gabon

Abstract

Objectives: Good-quality and sufficient DNA is essential for diagnostics and vaccine development. We aimed to compare six DNA extraction techniques applied to Loa loa microfilariae in order to evaluate the purity and integrity of extracts in terms of quality and quantity.

Methods: The microfilariae were purified via a Percoll gradient procedure with blood from hyper-microfilaremic individuals (> 30,000 microfilaria [mf]/ml). DNA extraction was carried out in duplicate at a rate of 350,000 mf/tube for each technique: phenol/chloroform, commercial Qiagen kit, salting out, Tris-EDTA, methanol, and cetyltrimethylammonium bromide (CTAB). The integrity, purity, concentration, and quality of the DNA extracts were successively verified by agarose gel electrophoresis, spectrophotometry (A260/A280 and A260/A230 wavelength ratio), Qubit fluorometry, and endonuclease and polymerase activity. The six techniques were compared on the basis of the following parameters: concentration, purity, efficiency, effectiveness, integrity, safety of the technique, as well as cost and duration of the protocol.

Results: The ratios of the optical densities of the extracts A260/A280 and A260/A230 were, respectively: phenol/chloroform (1.82; 1.11), Qiagen (1.93; 1.36), salting-out (1.9; 2.04), Tris-EDTA (1.99; 1.183), methanol (2.126; 1.343), and CTAB (2.01; 2.426). The DNA yield was: phenol/chloroform (3.920 μg), Qiagen (10.280 μg), salting-out (10.390 μg), Tris-EDTA (0.5528 μg), methanol (0.1036 μg), and CTAB (1.115 μg). Endonuclease and polymerase activity was demonstrated by digestion of DNA and through amplicons obtained via polymerase chain reaction assays with phenol/chloroform, Qiagen, and salting-out extracts.

Conclusion: The phenol/chloroform, Qiagen, and salting-out DNA extracts were all of good quality. Salting out had the best yield followed by Qiagen and then phenol/chloroform. Endonuclease and polymerase activity was effective in all three extracts despite the presence of some contaminants. These methods are therefore suitable for the extraction of DNA from Loa loa microfilariae. Tris-EDTA and methanol did not show adequate sensitivity, while CTAB was found to be unsuitable.

MeSH terms

Animals
Cetrimonium
Chloroform*
DNA / genetics
Edetic Acid
Endonucleases
Genomics
Humans
Loa* / genetics
Methanol
Phenol

Substances

Phenol
Chloroform
DNA
Edetic Acid
Endonucleases
Methanol
Cetrimonium

Grants and funding

The authors received no specific funding for this work.