Expanding the toolbox for molecular microbial studies: from communities to single cells
Recently, the molecular revolution and nanotechnologies have provided tools for
expanding the knowledge of microorganisms. This thesis had its starting point in
utilizing existing methods to identify specific microbes. Polymerase chain reaction
(PCR)-based assays were employed for the detection of zoonotic virus (Orthopoxvirus) in
capybara’s (Hydrochoerus hydrochaeris) faecal samples in an attempt to examine the
spread of viruses and a possible route for viral outbreaks. Here, the existing method was
sufficient to answer the question and find that viral genetic material is indeed present in
these stool samples. The established PCR and sequencing-based methods were also
applied to study bacteria responsible for the removal of highly chlorinated phenols from
contaminated sites. Despite detecting bacterial species from samples in situ or from
microcosm experiments, it became evident that the used method did not clarify which
microbes specifically were responsible for bioremediation. The abundance of
pentachlorophenol hydroxylase gene (pcpB), the major gene involved in the
bioremediation process, was detected with quantitative PCR and the overall bacterial
diversity with sequencing using the universal marker – the 16S rRNA gene. Yet, the real
players of the process remained unknown. This led to the quest to specify the
microorganisms that are carrying a specific gene. As a result, a novel method based on
droplet microfluidics technology was developed to investigate microbes at single-cell
resolution. Within these droplets, PCR is used to fuse 16S rRNA and a second gene of
interest into concatemers. Through sequencing, the second gene can be associated with
specific bacterial species. To make the method reliable, several individual steps in the
procedure required both engineering and careful method validation. These included the
elimination of errors stemming from the existence of DNA outside of the cells, the
efficient breaking of the emulsion and hence the collection of DNA, the blocking of
unwanted PCR amplification that was confounding the sequencing results, and ensuring
that the sample was studied at single-cell resolution. The established methods may be
applied to a variety of research where it is necessary to identify the microorganism
carriers of specific genetically encoded functions, and therefore highlight the potential
actors in the environmental processes.
Keywords: Methods in microbiology; NGS; PCR; single-cell technology; methods
in microbiology.
...
Publisher
Jyväskylän yliopistoISBN
978-951-39-8799-2ISSN Search the Publication Forum
2489-9003Contains publications
- Artikkeli I: Ambrosio Leal Dutra, L., Almeida, G. M. D. F., Oliveira, G. P., Abrahão, J. S., Kroon, E. G., & Trindade, G. D. S. (2017). Molecular evidence of Orthopoxvirus DNA in capybara (Hydrochoerus hydrochaeris) stool samples. Archives of Virology, 162(2), 439-448. DOI: 10.1007/s00705-016-3121-3
- Artikkeli II: Mikkonen, A., Yläranta, K., Tiirola, M., Ambrosio Leal Dutra, L., Salmi, P., Romantschuk, M., Copley, S., Ikäheimo, J., & Sinkkonen, A. (2018). Successful aerobic bioremediation of groundwater contaminated with higher chlorinated phenols by indigenous degrader bacteria. Water Research, 138, 118-128. DOI: 10.1016/j.watres.2018.03.033. JYX: jyx.jyu.fi/handle/123456789/57432
- Artikkeli III: Dutra, L., Franz, O., Puupponen, V.-M., & Tiirola, M. (2020). DNA recovery from Droplet Digital™ PCR emulsions using liquid nitrogen. Biotechniques, 69(9), 451-454. DOI: 10.2144/btn-2020-0076
- Artikkeli IV: Dutra, Lara; Jalasvuori, Matti; Franz, Ole; Salmi, Paulina; Nurminen, Kimi; Tiirola, Marja & Penttinen, Reetta (2021). Single-cell resolution genetic association analysis of heterogeneous bacterial communities by utilizing droplet digital PCR. Manuscript.
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- JYU Dissertations [871]
- Väitöskirjat [3599]
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