Summary of Study ST000875

This data is available at the NIH Common Fund's National Metabolomics Data Repository (NMDR) website, the Metabolomics Workbench, https://www.metabolomicsworkbench.org, where it has been assigned Project ID PR000606. The data can be accessed directly via it's Project DOI: 10.21228/M82D92 This work is supported by NIH grant, U2C- DK119886.

See: https://www.metabolomicsworkbench.org/about/howtocite.php

This study contains a large results data set and is not available in the mwTab file. It is only available for download via FTP as data file(s) here.

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Study ID	ST000875
Study Title	Metabolomic investigations on Nesterenkonia flava from different origins revealed significant intraspecies differences between marine and terrestrial actinomycetes
Study Summary	Marine is one of the most important resources of microorganisms, including bacteria, actinomycetes, and fungi. As marine and terrestrial environments differ a lot in many aspects it is not surprising that the species and characteristics of microorganisms living there are very different. Interestingly, many marine microorganisms can find their congeners of the same species from terrestrial resources. The aim of this work is to evaluate the intraspecies differences between marine and terrestrial actinomycetes on metabolic level and to uncover the mechanism responsible for the differences. To address this, we carried out comparative metabolomics study on Nesterenkonia flava strains isolated from marine and terrestrial environments. The results showed that marine strains were clearly distinguished from their terrestrial congeners on the principal components analysis (PCA) scores plot of intracellular metabolites. The markers responsible for the discrimination of marine and terrestrial strains were figured out using loading plot from partial least squares discrimination analysis (PLS-DA). Pathway analysis based on PLS-DA, univariate analysis, and correlation analysis of metabolites showed that the major differential metabolites between the terrestrial N. flava and the marine ones were involved in osmotic regulation, redox balancing, and energy metabolism. Together, these insights provide clues as to how the previous living environment of microbes affect their current metabolic performances under laboratory cultivation conditions.
Institute	Third Institute of Oceanography, State Oceanic Administration
Last Name	Xia
First Name	Jinmei
Address	184 Daxue Road, Xiamen 361005, PR China
Email	xiajinmei@tio.org.cn
Phone	86-13003995626
Submit Date	2017-08-12
Raw Data File Type(s)	fid
Analysis Type Detail	NMR
Release Date	2020-01-06
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR000606
Project DOI:	doi: 10.21228/M82D92
Project Title:	Metabolomic investigations on Nesterenkonia flava from different origins revealed significant intraspecies differences between marine and terrestrial actinomycetes
Project Summary:	Marine is one of the most important resources of microorganisms, including bacteria, actinomycetes, and fungi. As marine and terrestrial environments differ a lot in many aspects it is not surprising that the species and characteristics of microorganisms living there are very different. Interestingly, many marine microorganisms can find their congeners of the same species from terrestrial resources. The aim of this work is to evaluate the intraspecies differences between marine and terrestrial actinomycetes on metabolic level and to uncover the mechanism responsible for the differences. To address this, we carried out comparative metabolomics study on Nesterenkonia flava strains isolated from marine and terrestrial environments. The results showed that marine strains were clearly distinguished from their terrestrial congeners on the principal components analysis (PCA) scores plot of intracellular metabolites. The markers responsible for the discrimination of marine and terrestrial strains were figured out using loading plot from partial least squares discrimination analysis (PLS-DA). Pathway analysis based on PLS-DA, univariate analysis, and correlation analysis of metabolites showed that the major differential metabolites between the terrestrial N. flava and the marine ones were involved in osmotic regulation, redox balancing, and energy metabolism. Together, these insights provide clues as to how the previous living environment of microbes affect their current metabolic performances under laboratory cultivation conditions.
Institute:	Third Institute of Oceanography, State Oceanic Administration
Last Name:	Xia
First Name:	Jinmei
Address:	184 Daxue Road, Xiamen 361005, PR China
Email:	xiajinmei@tio.org.cn
Phone:	86-13003995626

Subject:

Subject ID:	SU001174
Subject Type:	NMR based metabolomics of microbes
Subject Species:	Nesterenkonia flava
Taxonomy ID:	469799

Factors:

Subject type: NMR based metabolomics of microbes; Subject species: Nesterenkonia flava (Factor headings shown in green)

mb_sample_id	local_sample_id	Strain	Strain source	Medium
SA077589	20	1A10663	Terrestrial	A14
SA077590	19	1A10663	Terrestrial	A14
SA077591	21	1A10663	Terrestrial	A14
SA077592	22	1A10663	Terrestrial	A14
SA077593	24	1A10663	Terrestrial	A14
SA077594	23	1A10663	Terrestrial	A14
SA077595	69	1A10663	Terrestrial	A3
SA077596	71	1A10663	Terrestrial	A3
SA077597	68	1A10663	Terrestrial	A3
SA077598	67	1A10663	Terrestrial	A3
SA077599	72	1A10663	Terrestrial	A3
SA077600	70	1A10663	Terrestrial	A3
SA077601	48	1A10663	Terrestrial	A6
SA077602	43	1A10663	Terrestrial	A6
SA077603	47	1A10663	Terrestrial	A6
SA077604	46	1A10663	Terrestrial	A6
SA077605	44	1A10663	Terrestrial	A6
SA077606	45	1A10663	Terrestrial	A6
SA077607	3	1K00606	Marine	A14
SA077608	2	1K00606	Marine	A14
SA077609	4	1K00606	Marine	A14
SA077610	1	1K00606	Marine	A14
SA077611	6	1K00606	Marine	A14
SA077612	5	1K00606	Marine	A14
SA077613	54	1K00606	Marine	A3
SA077614	53	1K00606	Marine	A3
SA077615	52	1K00606	Marine	A3
SA077616	51	1K00606	Marine	A3
SA077617	49	1K00606	Marine	A3
SA077618	50	1K00606	Marine	A3
SA077619	25	1K00606	Marine	A6
SA077620	27	1K00606	Marine	A6
SA077621	28	1K00606	Marine	A6
SA077622	26	1K00606	Marine	A6
SA077623	29	1K00606	Marine	A6
SA077624	30	1K00606	Marine	A6
SA077625	10	1K00607	Marine	A14
SA077626	11	1K00607	Marine	A14
SA077627	9	1K00607	Marine	A14
SA077628	7	1K00607	Marine	A14
SA077629	12	1K00607	Marine	A14
SA077630	8	1K00607	Marine	A14
SA077631	58	1K00607	Marine	A3
SA077632	56	1K00607	Marine	A3
SA077633	57	1K00607	Marine	A3
SA077634	55	1K00607	Marine	A3
SA077635	59	1K00607	Marine	A3
SA077636	60	1K00607	Marine	A3
SA077637	34	1K00607	Marine	A6
SA077638	31	1K00607	Marine	A6
SA077639	36	1K00607	Marine	A6
SA077640	32	1K00607	Marine	A6
SA077641	33	1K00607	Marine	A6
SA077642	35	1K00607	Marine	A6
SA077643	14	1K00610	Marine	A14
SA077644	13	1K00610	Marine	A14
SA077645	15	1K00610	Marine	A14
SA077646	16	1K00610	Marine	A14
SA077647	18	1K00610	Marine	A14
SA077648	17	1K00610	Marine	A14
SA077649	66	1K00610	Marine	A3
SA077650	65	1K00610	Marine	A3
SA077651	63	1K00610	Marine	A3
SA077652	61	1K00610	Marine	A3
SA077653	62	1K00610	Marine	A3
SA077654	64	1K00610	Marine	A3
SA077655	37	1K00610	Marine	A6
SA077656	38	1K00610	Marine	A6
SA077657	39	1K00610	Marine	A6
SA077658	40	1K00610	Marine	A6
SA077659	41	1K00610	Marine	A6
SA077660	42	1K00610	Marine	A6

Showing results 1 to 72 of 72

Showing results 1 to 72 of 72

Collection:

Collection ID:	CO001168
Collection Summary:	The broth cultures (50 mL) were harvested via centrifugation at 7000 g for 10 min under 4 °C. The pellet was quenched using 10 mL of 60% cold methanol (−80 °C) containing 0.85% (wt./vol.) of NaCl for 30 min. The quenched cell pellets were re-suspended in 10 mL of cold PBS and were washed for 3 times.
Sample Type:	Cultured cells

Treatment:

Treatment ID:	TR001188
Treatment Summary:	For each cell pellet sample, 5 mL of the mixture of methanol/water (1:0.9, v/v) was added and ultrasonicated for 25 min to break cells bathing in ice. The mixture was added with 5 mL of cold chloroform, vortexed and subjected to 10 min of ultrasonic extraction under the bath of ice. The mixture was then centrifuged at 9500 g for 8 min. The upper layer phase containing methanol and water was taken out and evaporated in the fume cupboard to remove methanol. The remaining water solution was freezed under −80 °C, and then freeze-dried to afford dry samples, which were stored under −80 °C before analysis.

Treatment ID:

TR001188

Treatment Summary:

For each cell pellet sample, 5 mL of the mixture of methanol/water (1:0.9, v/v) was added and ultrasonicated for 25 min to break cells bathing in ice. The mixture was added with 5 mL of cold chloroform, vortexed and subjected to 10 min of ultrasonic extraction under the bath of ice. The mixture was then centrifuged at 9500 g for 8 min. The upper layer phase containing methanol and water was taken out and evaporated in the fume cupboard to remove methanol. The remaining water solution was freezed under −80 °C, and then freeze-dried to afford dry samples, which were stored under −80 °C before analysis.

Sample Preparation:

Sampleprep ID:	SP001181
Sampleprep Summary:	The intracellular extract was re-suspended in 550 µL of phosphate buffer containing 1.5 M KH2PO4, 0.1% sodium 3-(trimethylsilyl) propionate-2,2,3,3-d4 (TSP), and 10% D2O. Subsequently, all the samples were vortexed and centrifuged at 12000 g for 15 min at 4°C to remove any insoluble components. The collected supernatants (500 μL) were transferred to 5 mm NMR tubes for analysis.

Analysis:

Analysis ID:	AN001828
Analysis Type:	NMR
Num Factors:	12

NMR:

NMR ID:	NM000141
Analysis ID:	AN001828
Instrument Name:	Bruker Avance III
Instrument Type:	FT-NMR
NMR Experiment Type:	1D 1H
Spectrometer Frequency:	850 MHz