Mosquito DNA Isolation and Species Identification

DNA isolation was performed from the whole mosquito body, except of the right wing. Individual specimens were placed into 2 ml tubes and about 10 pieces of 2.0 mm zirconia beads (BioSpec Products, Bartlesville, USA) as well as 1 ml of cell culture medium (high-glucose Dulbecco’s modified Eagle’s medium; Sigma-Aldrich, St. Louis, MO, USA) were added. The homogenization was performed with a Tissuelyser II (Qiagen, Hilden, Germany) for 2 min at 30 oscillations/s and 200 μl of the homogenate were used for DNA extraction, which was performed with KingFisher Flex Magnetic Particle Processor using MagMAX CORE Nucleic Acid Purification Kit (both Thermo Fisher Scientific, Waltham, MA, USA). Polymerase chain reaction (PCR) amplification of cytochrome oxidase subunit I (COI) gene region was conducted with the protocol published by Fang et al.^{32 (link)} using the primers by Folmer et al.³³. Sanger sequencing was applied for all positive amplicons (LGC Genomics, Berlin, Germany). Furthermore, morphologically identified Cx. pipiens s.l. and An. maculipennis s.l. specimens were typed to species level (Cx. pipiens pipiens form pipiens resp. Anopheles messeae) using two molecular assays^{34 (link),35 (link)}.

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Sauer F.G., Jaworski L., Erdbeer L., Heitmann A., Schmidt-Chanasit J., Kiel E, & Lühken R. (2020). Geometric morphometric wing analysis represents a robust tool to identify female mosquitoes (Diptera: Culicidae) in Germany. Scientific Reports, 10, 17613.

Publication 2020

high-glucose Dulbecco’s modified Eagle’s medium Tissuelyser II KingFisher Flex Magnetic Particle Processor MagMAX CORE Nucleic Acid Purification Kit

Anopheles Body Cell Cell culture Cytochrome oxidase Eagle Gene amplification Glucose Isolation Mosquito Nucleic acid Polymerase chain reaction Primers Resp Subunit Zirconia

Corresponding Organization : Carl von Ossietzky Universität Oldenburg

Other organizations : Bernhard Nocht Institute for Tropical Medicine

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Variable analysis

independent variables

DNA isolation method (whole mosquito body, except right wing)
Homogenization method (Tissuelyser II for 2 min at 30 oscillations/s)

dependent variables

DNA extraction yield
Successful PCR amplification of COI gene region
Sanger sequencing results

control variables

Mosquito species (Cx. pipiens s.l. and An. maculipennis s.l.)
Volume of cell culture medium (1 ml)
Number of zirconia beads (10 pieces of 2.0 mm)
DNA extraction method (KingFisher Flex Magnetic Particle Processor using MagMAX CORE Nucleic Acid Purification Kit)
PCR protocol (as published by Fang et al.)
Primer pairs (as used by Folmer et al.)

positive controls

Morphologically identified Cx. pipiens s.l. and An. maculipennis s.l. specimens
Molecular assays for species-level identification (Cx. pipiens pipiens form pipiens and Anopheles messeae)

negative controls

Not explicitly mentioned

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