Cutting corners: The impact of storage and DNA extraction on quality and quantity of DNA in honeybee (Apis mellifera) spermatheca

Ajda Moškrič; Anja Pavlin; Katarina Mole; Andraž Marinč; Jernej Bubnič; Andreja Opara; Marin Kovačić; Zlatko Puškadija; Aleksandar Uzunov; Sreten Andonov; Bjørn Dahle; Janez Prešern

doi:10.3389/fphys.2023.1139269

Cutting corners: The impact of storage and DNA extraction on quality and quantity of DNA in honeybee (Apis mellifera) spermatheca

Front Physiol. 2023 Mar 3:14:1139269. doi: 10.3389/fphys.2023.1139269. eCollection 2023.

Authors

Ajda Moškrič¹, Anja Pavlin^{1

2}, Katarina Mole¹, Andraž Marinč¹, Jernej Bubnič¹, Andreja Opara¹, Marin Kovačić^{3

4}, Zlatko Puškadija^{3

4}, Aleksandar Uzunov^{5

6}, Sreten Andonov⁷, Bjørn Dahle⁸, Janez Prešern¹

Affiliations

¹ Department of Animal Production, Agricultural Institute of Slovenia, Ljubljana, Slovenia.
² Department of Biology, Biotechnical faculty, University of Ljubljana, Ljubljana, Slovenia.
³ Faculty of Agrobiotechnical Sciences Osijek, University of J.J. Strossmayer, Osijek, Croatia.
⁴ Centre for Applied Life Sciences Healthy Food Chain Ltd., Osijek, Croatia.
⁵ Faculty of Agricultural Sciences and Food, Ss. Cyril and Methodius University in Skopje, Skopje, Macedonia.
⁶ Company for Applied Research and Permanent Education in Agriculture, Skopje, Macedonia.
⁷ Department of Animal Genetics, Swedish University of Agricultural Sciences, Uppsala, Sweden.
⁸ Norwegian Beekeepers Association, Kløfta, Norway.

Abstract

The purpose of our study was to investigate methods of short-term storage that allow preservation, transport and retrieval of genetic information contained in honeybee queen's spermatheca. Genotyping of the honeybee colony requires well ahead planned sample collection, depending on the type of data to be acquired. Sampling and genotyping of spermatheca's content instead of individual offspring is timesaving, allowing answers to the questions related to patriline composition immediately after mating. Such procedure is also cheaper and less error prone. For preservation either Allprotect Tissue Reagent (Qiagen) or absolute ethanol were used. Conditions during transportation were simulated by keeping samples 6-8 days at room temperature. Six different storing conditions of spermathecas were tested, complemented with two DNA extraction methods. We have analysed the concentration of DNA, RNA, and proteins in DNA extracts. We also analysed how strongly the DNA is subjected to fragmentation (through amplification of genetic markers ANT2 and tRNA^leu-COX2) and whether the quality of the extracted DNA is suitable for microsatellite (MS) analysis. Then, we tested the usage of spermatheca as a source of patriline composition in an experiment with three instrumentally inseminated virgin queens and performed MS analysis of the extracted DNA from each spermatheca, as well as queens' and drones' tissue. Our results show that median DNA concentration from spermathecas excised prior the storage, regardless of the storing condition and DNA extraction method, were generally lower than median DNA concentration obtained from spermathecas dissected from the whole queens after the storage. Despite the differences in DNA yield from the samples subjected to different storing conditions there was no significant effect of storage method or the DNA extraction method on the amplification success, although fewer samples stored in EtOH amplified successfully in comparison to ATR storing reagent. However, we recommend EtOH as a storing reagent due to its availability, low price, simplicity in usage in the field and in the laboratory, and capability of good preservation of the samples for DNA analysis during transport at room temperature.

Keywords: Apis mellifera; DNA extraction; breeding; honeybee; microsatellite; patriline; preservation method; spermatheca.

Grants and funding

This research was funded by ARRS Research Programs (P4-0133 Sustainable agriculture, AMa, KM, AMo, and AO; P4-0431 NextGenAgri, JP and JB), through ARRS Applied Research Project (L4-2624, co-financed by ARRS and MKGP; JP, AMo, KM and AMa), through Young researcher’s grant 1000-20-0401 (JB) and EEA and Norway Grants Fund for Regional Cooperation project BeeConSel, Grant No. 2018-1-0477 (JP, AMo, KM, AMa, MK, ZP, AU, SA, AP, and BD).