Abstract
AbstractCounting viable cells is a universal practice in microbiology. The colony forming unit (CFU) assay has remained the gold standard to measure viability across disciplines; however, it is time-intensive and resource-consuming. Herein, we describe the Geometric Viability Assay (GVA) that replicates CFU measurements over 6-orders of magnitude while reducing over 10-fold the time and consumables. GVA computes a sample’s viable cell count based on the distribution of embedded colonies growing inside a pipette tip. GVA is compatible with gram-positive and -negative planktonic bacteria, biofilms, and yeast. Laborious CFU experiments such as checkerboard assays, treatment time-courses, and drug screens against slow-growing cells are simplified by GVA. We therefore screened a drug library against exponential and stationary phaseE. colileading to the discovery of the ROS-mediated, bactericidal mechanism of diphenyliodonium. The ease and low cost of GVA evinces it can accelerate existing viability assays and enable measurements at previously impractical scales.
Publisher
Cold Spring Harbor Laboratory
Reference43 articles.
1. Lázár, V. , Snitser, O. , Barkan, D. & Kishony, R. Antibiotic combinations reduce Staphylococcus aureus clearance. Nature, 1–7 (Oct. 2022).
2. Eradicating Bacterial Persisters with Combinations of Strongly and Weakly Metabolism-Dependent Antibiotics;Cell chemical biology,2020
3. Hazan, R. , Que, Y. A. , Maura, D. & Rahme, L. G. A method for high throughput determination of viable bacteria cell counts in 96-well plates. BMC Microbiology 12 (Nov. 2012).
4. Adaptation of the Start-Growth-Time Method for High-Throughput Biofilm Quantification;Frontiers in Microbiology,2021
5. Assessing Pseudomonas aeruginosa Persister/antibiotic tolerant cells;Methods in molecular biology,2014