Immobilization of Phosphatidylserine by Ethanol and Lysozyme on the Cell Surface for Evaluation of Apoptosis-Like Decay in Activated-Sludge Bacteria

Ben Chen; Yasi Zhao; Zemin Li; Jianxin Pan; Haizhen Wu; Guanglei Qiu; Chunhua Feng; Chaohai Wei

doi:10.1128/AEM.00345-20

Immobilization of Phosphatidylserine by Ethanol and Lysozyme on the Cell Surface for Evaluation of Apoptosis-Like Decay in Activated-Sludge Bacteria

Appl Environ Microbiol. 2020 Jul 2;86(14):e00345-20. doi: 10.1128/AEM.00345-20. Print 2020 Jul 2.

Authors

Ben Chen¹, Yasi Zhao¹, Zemin Li¹, Jianxin Pan¹, Haizhen Wu², Guanglei Qiu^{1

3}, Chunhua Feng^{1

3}, Chaohai Wei^{4

3}

Affiliations

¹ School of Environment and Energy, South China University of Technology, Guangzhou, People's Republic of China.
² School of Biology and Biological Engineering, South China University of Technology, Guangzhou, People's Republic of China.
³ Key Laboratory of Pollution Control and Ecosystem Restoration in Industry Clusters, Ministry of Education, South China University of Technology, Guangzhou, People's Republic of China.
⁴ School of Environment and Energy, South China University of Technology, Guangzhou, People's Republic of China cechwei@scut.edu.cn.

Abstract

Accurate determination of microbial viability can be crucial in microbe-dominated biosystems. However, the identification of metabolic decay in bacterial cells can be elaborate and difficult. We sought to identify apoptosis-like bacterial processes by using annexin V-fluorescein isothiocyanate (FITC) (AVF), a probe typically used to stain phosphatidylserine (PS) on exposed cell membranes. The bacterial cell wall provides a barrier that is responsible for low efficiency of direct PS staining of decayed bacterial cells. This can be overcome by pretreatment of the bacteria with 70% ethanol, which fixates the bacteria and preserves the PS status, combined with lysozyme treatment to hydrolyze the cell wall. That treatment improved the efficiency of AVF staining considerably, as shown for pure strains of an Ochrobactrum sp. and a Micrococcus sp. Using this method, decayed bacterial cells (induced by starvation) were more strongly stained, indicating externalization of PS to a greater extent than seen for cells harvested at logarithmic growth. A multispecies microbial sludge was artificially decayed by heat treatment or alternating anoxic-oxic treatment, which also induced increased AVF staining, again presumably via decay-related PS externalization. The method developed proved to be efficient for identification of bacterial decay and has potential for the evaluation of multispecies bacterial samples from sources like soil matrix, bioaerosol, and activated sludge.IMPORTANCE Since the externalization of phosphatidylserine (PS) is considered a crucial characteristic of apoptosis, we sought to identify apoptosis-like decay in bacterial cells by PS staining using AVF. We show that this is possible, provided the bacteria are pretreated with ethanol plus lysozyme to remove a physical staining barrier and preserve the original, decay-related externalization of PS. Our work suggests that PS externalization occurs in starved bacteria and this can be quantified with AVF staining, providing a measure of bacterial decay. Since PS is the common component of the lipid bilayer in bacterial cell membranes, this approach also has potential for evaluation of cell decay of other bacterial species.

Keywords: activated sludge; annexin V-FITC staining; apoptosis-like decay; bacterial viability; ethanol-lysozyme treatment.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Apoptosis
Cell Wall / physiology
Ethanol / metabolism*
Micrococcus / metabolism*
Muramidase / metabolism*
Ochrobactrum / metabolism*
Phosphatidylserines / metabolism*
Sewage / microbiology

Substances

Phosphatidylserines
Sewage
Ethanol
Muramidase