The direct inhibitory effects of Lactobacillus acidophilus, a commensal urinary bacterium, on calcium oxalate stone development

Noonin C.; Putpim A.; Thongboonkerd V.

The direct inhibitory effects of Lactobacillus acidophilus, a commensal urinary bacterium, on calcium oxalate stone development

Issued Date

2024-12-01

Resource Type

Article

eISSN

20492618

DOI

10.1186/s40168-024-01877-y

Scopus ID

2-s2.0-85204219033

Journal Title

Microbiome

Volume

12

Issue

1

Rights Holder(s)

SCOPUS

Bibliographic Citation

Microbiome Vol.12 No.1 (2024)

Suggested Citation

Noonin C., Putpim A., Thongboonkerd V. The direct inhibitory effects of Lactobacillus acidophilus, a commensal urinary bacterium, on calcium oxalate stone development. Microbiome Vol.12 No.1 (2024). doi:10.1186/s40168-024-01877-y Retrieved from: https://repository.li.mahidol.ac.th/handle/20.500.14594/101337

Title

The direct inhibitory effects of Lactobacillus acidophilus, a commensal urinary bacterium, on calcium oxalate stone development

Author(s)

Noonin C.
Putpim A.
Thongboonkerd V.

Author's Affiliation

Siriraj Hospital

Corresponding Author(s)

Noonin C.

Other Contributor(s)

Mahidol University

Abstract

Background: Lactobacillus acidophilus is a commensal urinary bacterium found more abundantly in healthy individuals than in stone patients. Hence, it has been proposed to play an inhibitory role in kidney stone disease (KSD) but with unclear mechanisms. We therefore investigated the direct effects of L. acidophilus on calcium oxalate (CaOx) stone development compared with Escherichia coli, which is known to promote CaOx stone formation. Results: L. acidophilus at 1 × 103 CFU/ml significantly reduced the abundance of newly formed crystals, enlargement and aggregation of seeded crystals, and crystal adhesion on renal cell membranes. By contrast, E. coli at 1 × 103 CFU/ml significantly enhanced crystal growth and aggregation but did not affect crystallization and crystal-cell adhesion. Oxalate consumption assay showed that neither L. acidophilus nor E. coli significantly reduced the remaining oxalate level after 1 − 3 h incubation. However, both of them adhered to CaOx crystals. Surface component detection revealed that only L. acidophilus expressed S-layer protein, whereas only E. coli exhibited flagella on their surfaces. Removal of L. acidophilus S-layer protein and E. coli flagella completely abolished the inhibitory and promoting effects of L. acidophilus and E. coli, respectively. Conclusions: L. acidophilus inhibits CaOx stone development by hampering crystallization, growth, aggregation and cell-adhesive ability of CaOx. By contrast, E. coli enhances CaOx stone development by promoting CaOx growth and aggregation. Their contradictory effects are most likely from differential surface components (i.e., S-layer protein on L. acidophilus and flagella on E. coli) not from oxalate-degrading ability. D_jrSVq7xgjsSvuNUfqm6AVideo Abstract

Keyword(s)

Medicine
Immunology and Microbiology

URI

https://repository.li.mahidol.ac.th/handle/20.500.14594/101337

Collections

Scopus 2024

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