Summary of Study ST001633

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 PR001031. The data can be accessed directly via it's Project DOI: 10.21228/M8F39C This work is supported by NIH grant, U2C- DK119886.

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

Study ID	ST001633
Study Title	Aromatic amino acid metabolism by the anaerobic gut bacterium Clostridium sporogenes (part-II)
Study Summary	Germ-free MCAD-/- mice or MCAD+/+ controls were mono-colonized with wild-type Clostridium sporogenes. Urine was collected for untargeted LC-QTOF analysis.
Institute	Stanford University
Laboratory	Dodd
Last Name	Pruss
First Name	Kali
Address	300 Pasteur Drive, Lane 235
Email	kmpruss@stanford.edu
Phone	6507212961
Submit Date	2020-12-11
Raw Data Available	Yes
Raw Data File Type(s)	d
Analysis Type Detail	LC-MS
Release Date	2021-01-26
Release Version	1

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Project:

Project ID:	PR001031
Project DOI:	doi: 10.21228/M8F39C
Project Title:	Metabolic interactions between gut microbiota and the mammalian host
Project Summary:	Untargeted metabolomics performed on various host compartments under different colonization states in gnotobiotic mice.
Institute:	Stanford University
Laboratory:	Dodd
Last Name:	Pruss
First Name:	Kali
Address:	300 Pasteur Drive, Lane 235
Email:	kmpruss@stanford.edu
Phone:	6507212961

Subject:

Subject ID:	SU001710
Subject Type:	Mammal
Subject Species:	Mus musculus
Taxonomy ID:	10090

Factors:

Subject type: Mammal; Subject species: Mus musculus (Factor headings shown in green)

mb_sample_id	local_sample_id	Mouse_Genotype	Treatment
SA138160	18	MCAD+/+	Cs
SA138161	17	MCAD+/+	Cs
SA138162	16	MCAD+/+	Cs
SA138163	19	MCAD+/+	Cs
SA138164	20	MCAD+/+	Cs
SA138165	22	MCAD+/+	Cs
SA138166	21	MCAD+/+	Cs
SA138167	12	MCAD+/+	Cs
SA138168	11	MCAD+/+	Cs
SA138169	10	MCAD+/+	Cs
SA138170	9	MCAD+/+	Cs
SA138185	36	MCAD-/-	Cs
SA138186	35	MCAD-/-	Cs
SA138187	37	MCAD-/-	Cs
SA138188	39	MCAD-/-	Cs
SA138189	34	MCAD-/-	Cs
SA138190	24	MCAD-/-	Cs
SA138191	38	MCAD-/-	Cs
SA138192	15	MCAD-/-	Cs
SA138193	33	MCAD-/-	Cs
SA138194	14	MCAD-/-	Cs
SA138195	13	MCAD-/-	Cs
SA138196	23	MCAD-/-	Cs
SA138171	31	MCAD+/+	GF
SA138172	32	MCAD+/+	GF
SA138173	40	MCAD+/+	GF
SA138174	41	MCAD+/+	GF
SA138175	30	MCAD+/+	GF
SA138176	29	MCAD+/+	GF
SA138177	27	MCAD+/+	GF
SA138178	1	MCAD+/+	GF
SA138179	25	MCAD+/+	GF
SA138180	28	MCAD+/+	GF
SA138181	26	MCAD+/+	GF
SA138182	4	MCAD+/+	GF
SA138183	3	MCAD+/+	GF
SA138184	2	MCAD+/+	GF
SA138197	48	MCAD-/-	GF
SA138198	49	MCAD-/-	GF
SA138199	52	MCAD-/-	GF
SA138200	47	MCAD-/-	GF
SA138201	51	MCAD-/-	GF
SA138202	50	MCAD-/-	GF
SA138203	44	MCAD-/-	GF
SA138204	6	MCAD-/-	GF
SA138205	5	MCAD-/-	GF
SA138206	7	MCAD-/-	GF
SA138207	8	MCAD-/-	GF
SA138208	45	MCAD-/-	GF
SA138209	43	MCAD-/-	GF
SA138210	46	MCAD-/-	GF

Showing results 1 to 51 of 51

Showing results 1 to 51 of 51

Collection:

Collection ID:	CO001703
Collection Summary:	MCAD-/- mice were re-derived as germ-free (GF) for the purpose of this study. MCAD-/- mice or MCAD+/+ controls were maintained in sterile gnotobiotic isolators or cages with HEPA-filtered air supply. Urine from GF MCAD-/- and MCAD+/+ mice was collected under sterile conditions. Seven days subsequent, mice were mono-colonized with wild-type C. sporogenes (Cs) by gavage of 200 µL saturated overnight culture. Urine was collected one week after colonization. C. sporogenes colonization was verified with serial dilution plating. Urine samples were immediately frozen on dry ice and stored under -80 oC until analysis.
Sample Type:	Urine
Storage Conditions:	-80℃

Treatment:

Treatment ID:	TR001723
Treatment Summary:	MCAD-/- mice were re-derived as germ-free (GF) for the purpose of this study. MCAD-/- mice or MCAD+/+ controls were maintained in sterile gnotobiotic isolators or cages with HEPA-filtered air supply. Urine from GF MCAD-/- and MCAD+/+ mice was collected under sterile conditions. Seven days subsequent, mice were mono-colonized with wild-type C. sporogenes (Cs) by gavage of 200 µL saturated overnight culture. Urine was collected one week after colonization. C. sporogenes colonization was verified with serial dilution plating.

Treatment ID:

TR001723

Treatment Summary:

MCAD-/- mice were re-derived as germ-free (GF) for the purpose of this study. MCAD-/- mice or MCAD+/+ controls were maintained in sterile gnotobiotic isolators or cages with HEPA-filtered air supply. Urine from GF MCAD-/- and MCAD+/+ mice was collected under sterile conditions. Seven days subsequent, mice were mono-colonized with wild-type C. sporogenes (Cs) by gavage of 200 µL saturated overnight culture. Urine was collected one week after colonization. C. sporogenes colonization was verified with serial dilution plating.

Sample Preparation:

Sampleprep ID:	SP001716
Sampleprep Summary:	. Mouse urine samples (2.5 μL) were diluted with LC-MS grade water (5 μL) and mixed with internal standard (7.5 μL, d3-creatinine,1 mM; d9-phenylpropionic acid, 0.2 mM; 2,2-d2-hippuric acid, 0.2 mM), then 60 μL of extraction solvent containing reference standards (d7-glucose, d3-methionine, L-4-hydroxyphenyl-d4-alanine, d5-hippuric acid, d5-tryptophan, d3-leucine, di-n-octyl phthalate-3,4,5,6-d4, d19-decanoic acid, d15-octanoic acid, d27-tetradecanoic acid, 2-flurophenylglycine, d9-carnitine in methanol) was added to precipitate proteins. The solution was vortexed, then the plate was centrifuged at 15,000 x g for 5 min at 4 C. Supernatant (60 μL) was transferred to a new plate and 20 μL of each was diluted with 60 μL LC-MS grade water. Three procedure blanks were included using the same preparation method with LC-MS water (2.5 μL) instead of urine sample. Quality controls (QC) were pooled from each LC-MS ready sample.

Sampleprep ID:

SP001716

Sampleprep Summary:

. Mouse urine samples (2.5 μL) were diluted with LC-MS grade water (5 μL) and mixed with internal standard (7.5 μL, d3-creatinine,1 mM; d9-phenylpropionic acid, 0.2 mM; 2,2-d2-hippuric acid, 0.2 mM), then 60 μL of extraction solvent containing reference standards (d7-glucose, d3-methionine, L-4-hydroxyphenyl-d4-alanine, d5-hippuric acid, d5-tryptophan, d3-leucine, di-n-octyl phthalate-3,4,5,6-d4, d19-decanoic acid, d15-octanoic acid, d27-tetradecanoic acid, 2-flurophenylglycine, d9-carnitine in methanol) was added to precipitate proteins. The solution was vortexed, then the plate was centrifuged at 15,000 x g for 5 min at 4 C. Supernatant (60 μL) was transferred to a new plate and 20 μL of each was diluted with 60 μL LC-MS grade water. Three procedure blanks were included using the same preparation method with LC-MS water (2.5 μL) instead of urine sample. Quality controls (QC) were pooled from each LC-MS ready sample.

Combined analysis:

Analysis ID	AN002669
Analysis type	MS
Chromatography type	Reversed phase
Chromatography system	Agilent 1290 Infinity II UPLC
Column	Waters BEH C18 (100 x 2.1mm,1.7um)
MS Type	ESI
MS instrument type	QTOF
MS instrument name	Agilent 6545XT QTOF
Ion Mode	UNSPECIFIED
Units	peak height normalized with creatinine

Chromatography:

Chromatography ID:	CH001964
Instrument Name:	Agilent 1290 Infinity II UPLC
Column Name:	Waters BEH C18 (100 x 2.1mm,1.7um)
Chromatography Type:	Reversed phase

MS:

MS ID:	MS002468
Analysis ID:	AN002669
Instrument Name:	Agilent 6545XT QTOF
Instrument Type:	QTOF
MS Type:	ESI
MS Comments:	Acquisition was done in All-Ions fragmentation mode using collision energies of 0, 20, and 40 eV. Suspect screening was performed with MS-DIAL (version 4.24) and MS-CleanR. Peak height was normalized with creatinine
Ion Mode:	UNSPECIFIED