Evaluation of female Aedes aegypti proteome via LC-ESI-MS/MS using two protein extraction methods

Author:

Shettima Abubakar12,Ishak Intan H.34,Abdul Rais Syahirah Hanisah1,Abu Hasan Hadura34,Othman Nurulhasanah1

Affiliation:

1. Institute for Research in Molecular Medicine (INFORMM), Universiti Sains Malaysia, Gelugor, Pulau Pinang, Malaysia

2. Department of Microbiology, Faculty of Science, University of Maiduguri, Maiduguri, Borno State, Nigeria

3. School of Biological Sciences, Universiti Sains Malaysia, Gelugor, Pulau Pinang, Malaysia

4. Vector Control Research Unit (VCRU), School of Biological Sciences, Universiti Sains Malaysia, Gelugor, Pulau Pinang, Malaysia

Abstract

Background Proteomic analyses have broadened the horizons of vector control measures by identifying proteins associated with different biological and physiological processes and give further insight into the mosquitoes’ biology, mechanism of insecticide resistance and pathogens-mosquitoes interaction. Female Ae. aegypti ingests human blood to acquire the requisite nutrients to make eggs. During blood ingestion, female mosquitoes transmit different pathogens. Therefore, this study aimed to determine the best protein extraction method for mass spectrometry analysis which will allow a better proteome profiling for female mosquitoes. Methods In this present study, two protein extractions methods were performed to analyze female Ae. aegyti proteome, via TCA acetone precipitation extraction method and a commercial protein extraction reagent CytoBusterTM. Then, protein identification was performed by LC-ESI-MS/MS and followed by functional protein annotation analysis. Results The CytoBusterTM reagent gave the highest protein yield with a mean of 475.90 µg compared to TCA acetone precipitation extraction showed 283.15 µg mean of protein. LC-ESI-MS/MS identified 1,290 and 890 proteins from the CytoBusterTM reagent and TCA acetone precipitation, respectively. When comparing the protein class categories in both methods, there were three additional categories for proteins identified using CytoBusterTM reagent. The proteins were related to scaffold/adaptor protein (PC00226), protein binding activity modulator (PC00095) and intercellular signal molecule (PC00207). In conclusion, the CytoBusterTM protein extraction reagent showed a better performance for the extraction of proteins in term of the protein yield, proteome coverage and extraction speed.

Funder

Universiti Sains Malaysia, Research University Individual Grant

Publisher

PeerJ

Subject

General Agricultural and Biological Sciences,General Biochemistry, Genetics and Molecular Biology,General Medicine,General Neuroscience

Reference16 articles.

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