volume 70 issue 1 pages 8

Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal

Publication typeJournal Article
Publication date2025-02-07
scimago Q4
SJR0.105
CiteScore0.2
Impact factor
ISSN04389573, 24594113, 28139054
Abstract

In our previous study, Lentzea sp. JNUCC 0626 was isolated from Hwasun Gotjawal on Jeju Island, and its melanogenic effects were confirmed in B16F10 melanoma cells through the identification of 1-acetyl-β-carboline. In this study, we conducted a comprehensive taxonomic characterization of Lentzea sp. JNUCC 0626, including enzymatic activities, carbohydrate metabolism, growth conditions, and cellular composition. Major fatty acids identified were iso-C16:0, iso-C15:0, and C15:0 anteiso, with polar lipids such as diphosphatidylglycerol, phosphatidylethanolamine, and several unidentified lipids. Ubiquinone Q-9 was determined as the predominant respiratory quinone. Enzymatic activity analysis (API ZYM) showed alkaline phosphatase, esterase (C4), esterase lipase (C8), and leucine arylamidase activities, while carbohydrate metabolism analysis (API 50CHB) indicated acid production from esculin alone. Complete genome sequencing revealed a 10,602,950 bp linear chromosome and a 177,940 bp plasmid. This plasmid encodes essential plasmid-related genes, including a Type IV secretion system and ParA proteins critical for plasmid transfer and stability. These findings suggest that the plasmid in Lentzea sp. JNUCC 0626 could be utilized for developing host–vector systems to facilitate the combinatorial biosynthesis of novel bioactive compounds. Comparative genomic analysis identified Lentzea pudingi CGMCC 4.7319 as the closest relative, but significant genetic divergence (dDDH 46.7%, ANI 88.02%) strongly supports the classification of Lentzea sp. JNUCC 0626 as a novel species. AntiSMASH analysis revealed 34 biosynthetic gene clusters (BGCs), highlighting the strain’s capacity to produce diverse bioactive compounds. Finally, the JNUCC 0626 extract exhibited concentration-dependent NO inhibition in LPS-stimulated RAW 264.7 cells, demonstrating significant anti-inflammatory activity. This suggests that the secondary metabolites inferred from genomic analysis may contribute to these observed bioactivities.

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Hyun K., Boo K. H., Hyun C. D. Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal // Acta Microbiologica Hellenica. 2025. Vol. 70. No. 1. p. 8.
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Hyun K., Boo K. H., Hyun C. D. Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal // Acta Microbiologica Hellenica. 2025. Vol. 70. No. 1. p. 8.
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TY - JOUR
DO - 10.3390/amh70010008
UR - https://www.mdpi.com/2813-9054/70/1/8
TI - Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal
T2 - Acta Microbiologica Hellenica
AU - Hyun, Kyung-A
AU - Boo, Kyung Hwan
AU - Hyun, Chang Dong
PY - 2025
DA - 2025/02/07
PB - MDPI
SP - 8
IS - 1
VL - 70
SN - 0438-9573
SN - 2459-4113
SN - 2813-9054
ER -
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@article{2025_Hyun,
author = {Kyung-A Hyun and Kyung Hwan Boo and Chang Dong Hyun},
title = {Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal},
journal = {Acta Microbiologica Hellenica},
year = {2025},
volume = {70},
publisher = {MDPI},
month = {feb},
url = {https://www.mdpi.com/2813-9054/70/1/8},
number = {1},
pages = {8},
doi = {10.3390/amh70010008}
}
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Hyun, Kyung-A, et al. “Taxonomic Identification, Complete Genome Sequencing, and In Silico Genome Mining of the Actinobacterium Lentzea sp. JNUCC 0626 Isolated from Jeju Gotjawal.” Acta Microbiologica Hellenica, vol. 70, no. 1, Feb. 2025, p. 8. https://www.mdpi.com/2813-9054/70/1/8.