Detection and cell sorting of Pseudonocardia species by fluorescence in situ hybridization and flow cytometry using 16S rRNA-targeted oligonucleotide probes

Authors

Mengyan Li, New Jersey Institute of Technology
Yu Yang, George R. Brown School of Engineering and Computing
Ya He, George R. Brown School of Engineering and Computing
Jacques Mathieu, George R. Brown School of Engineering and Computing
Cong Yu, George R. Brown School of Engineering and Computing
Qilin Li, George R. Brown School of Engineering and Computing
Pedro J.J. Alvarez, George R. Brown School of Engineering and Computing

Document Type

Article

Publication Date

4-1-2018

Abstract

Pseudonocardia spp. are receiving increasing attention due to their ability to biodegrade recalcitrant cyclic ether pollutants (e.g., 1,4-dioxane and tetrahydrofuran), as well as for their distinctive ecological niches (e.g., symbiosis with ants/plants and production of antibiotics). Isolating and characterizing Pseudonocardia spp. is thus important to discern their metabolic and physiological idiosyncrasies and advance their potential applications. However, slow growth, low cell yield, and dissimilar colony morphology hinder efficient isolation of Pseudonocardia using conventional plating methods. Here, we develop the first fluorescent probe (Pse631) targeting the 16S rRNA of Pseudonocardia members. In combination with flow cytometry and cell sorting, in situ hybridization with this probe enables sensitive and specific detection of Pseudonocardia cells in mixed cultures and enriched environmental samples without significant false positives, using Escherichia coli, Bacillus subtilis, and Mycobacterium spp. as negative controls. Pseudonocardia dioxanivorans CB1190 cells labeled with Pse631 as a positive control were detected when their relative abundance in the total bacterial community was as low as 0.1%. Effective separation of Pseudonocardia cells from the mixed consortium was confirmed by quantitative PCR analysis of sorted cells. This study provides a culture-independent high-throughput molecular approach enabling effective separation of Pseudonocardia populations from complex microbial communities. This approach will not only facilitate subsequent molecular analyses including species identification and quantification, but also advance understanding of their catabolic capacities and functional molecular diversity.

Identifier

85042230940 (Scopus)

Publication Title

Applied Microbiology and Biotechnology

External Full Text Location

https://doi.org/10.1007/s00253-018-8801-3

e-ISSN

14320614

ISSN

01757598

PubMed ID

29464325

First Page

3375

Last Page

3386

Issue

7

Volume

102

Grant

ER-2301

Recommended Citation

Li, Mengyan; Yang, Yu; He, Ya; Mathieu, Jacques; Yu, Cong; Li, Qilin; and Alvarez, Pedro J.J., "Detection and cell sorting of Pseudonocardia species by fluorescence in situ hybridization and flow cytometry using 16S rRNA-targeted oligonucleotide probes" (2018). Faculty Publications. 8744.
https://digitalcommons.njit.edu/fac_pubs/8744