Improving the Accuracy of Flow Cytometric Quantification of Microbial Populations in Sediments: Importance of Cell Staining Procedures

Longhui Deng; Annika Fiskal; Xingguo Han; Nathalie Dubois; Stefano Michele Bernasconi; Mark Alexander Lever

doi:10.3389/fmicb.2019.00720

Improving the Accuracy of Flow Cytometric Quantification of Microbial Populations in Sediments: Importance of Cell Staining Procedures

Front Microbiol. 2019 Apr 9:10:720. doi: 10.3389/fmicb.2019.00720. eCollection 2019.

Authors

Longhui Deng¹, Annika Fiskal¹, Xingguo Han¹, Nathalie Dubois^{2

3}, Stefano Michele Bernasconi³, Mark Alexander Lever¹

Affiliations

¹ Institute of Biogeochemistry and Pollutant Dynamics, ETH Zürich, Zurich, Switzerland.
² Surface Waters Research-Management, Eawag, Swiss Federal Institute of Aquatic Science and Technology, Dübendorf, Switzerland.
³ Department of Earth Sciences, ETH Zürich, Zurich, Switzerland.

Abstract

The accuracy of flow cytometric (FCM) quantifications of microbial populations in sediments varies with FCM settings, cell extraction and staining protocols, as well as sample types. In the present study, we improve the accuracy of FCM for enumerating microorganisms inhabiting diverse lake and marine sediment types based on extensive tests with FCM settings, extraction buffer chemical compositions, cell separation methods, and staining procedures. Tests on the FCM settings, (e.g., acquisition time, rates of events) and salinity of extraction solutions show minor impacts on FCM enumerations and yields of cell extraction, respectively. Existing methods involving hydrofluoric acid (HF) treatment to release sediment-attached cells into solution prove effective on both marine and freshwater samples. Yet, different staining techniques (direct staining of cell extracts, staining of membrane-filtered cell extracts) produce clear differences in cell number estimates. We demonstrate that, while labor-intensive membrane-staining generates high cell staining efficiency and accurate cell counts that are consistent across FCM and epifluorescence microscopy-based (EFM) quantification methods, accurate cell counts determined by more time- and labor-efficient direct staining require consideration of dye concentration, sample dilution, and lithology. Yet, good agreement between the two staining methods can be achieved through sample-specific adjustments of dye concentrations and sample dilutions during direct staining. We thus present a complete protocol for FCM-based cell quantification, that includes all steps from the initial sample fixation to the final enumeration, with recommendations for buffer compositions, direct and membrane-based staining procedures, and the final FCM assay. This protocol is versatile, accurate, and reliable, as is evident from good agreement with cell quantifications by EFM and quantitative polymerase chain reaction (qPCR) of 16S rRNA genes across a wide range of sedimentary sample types.

Keywords: cell counts; epifluorescence microscopy; flow cytometry; lacustrine; marine; microbial populations; staining technique.