Summary of Study ST002442

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 PR001573. The data can be accessed directly via it's Project DOI: 10.21228/M8CD9V 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 IDST002442
Study TitleAlterations in CSF Urea Occur in Late Manifest Stage Huntington Disease
Study Typeuntargeted metabolomics analysis
Study SummaryHuntington Disease (HD) is a neurodegenerative disorder caused by expanded cytosine-adenine-guanine (CAG) repeats in the Huntingtin gene, resulting in the production of mutant huntingtin proteins (mHTT). Previous research has identified urea as a key metabolite elevated in HD animal models and post-mortem tissues of HD patients. The exact timing of these elevations in urea and the molecular mechanism(s) responsible for these disturbances remain unknown. To better understand the pathophysiologic mechanisms responsible for elevations in urea in HD, we completed a global metabolomic profile of cerebrospinal fluid (CSF) from individuals who were at several stages of disease: pre-manifest (PRE), manifest (MAN), and late-manifest (LATE) HD participants compared to controls. We found approximately 500 metabolites were significantly altered in pre-manifest participants compared to controls, although no significant difference in CSF urea or urea metabolites. Interestingly, CSF urea was only significantly elevated in LATE participants compared to controls. There were no changes in the urea metabolites, citrulline, ornithine and arginine throughout disease; however, we did observe changes in acetate, creatinine, 4-acetamidobutanoate and 4-aminobutyraldehyde which are indirect modifiers of urea. Overall, our study confirms that elevations in urea do occur in HD, albeit later in disease and that these changes may reflect more central impairments to cellular energy metabolism yet to be explored.
Institute
Vanderbilt University
DepartmentChemistry
LaboratoryCenter for Innovative Technology
Last NameCODREANU
First NameSIMONA
Address1234 STEVENSON CENTER LANE
EmailSIMONA.CODREANU@VANDERBILT.EDU
Phone6158758422
Submit Date2023-01-12
Num Groups4
Total Subjects60
Raw Data AvailableYes
Raw Data File Type(s)raw(Thermo)
Analysis Type DetailLC-MS
Release Date2023-01-25
Release Version1
SIMONA CODREANU SIMONA CODREANU
https://dx.doi.org/10.21228/M8CD9V
ftp://www.metabolomicsworkbench.org/Studies/ application/zip

Select appropriate tab below to view additional metadata details:

Project:

Project ID:PR001573
Project DOI:doi: 10.21228/M8CD9V
Project Title:Alterations in CSF Urea Occur in Late Manifest Stage Huntington Disease
Project Type:Untargeted Metabolomics analysis
Project Summary:Huntington Disease (HD) is a neurodegenerative disorder caused by expanded cytosine-adenine-guanine (CAG) repeats in the Huntingtin gene, resulting in the production of mutant huntingtin proteins (mHTT). Previous research has identified urea as a key metabolite elevated in HD animal models and post-mortem tissues of HD patients. The exact timing of these elevations in urea and the molecular mechanism(s) responsible for these disturbances remain unknown. To better understand the pathophysiologic mechanisms responsible for elevations in urea in HD, we completed a global metabolomic profile of cerebrospinal fluid (CSF) from individuals who were at several stages of disease: pre-manifest (PRE), manifest (MAN), and late-manifest (LATE) HD participants compared to controls. We found approximately 500 metabolites were significantly altered in pre-manifest participants compared to controls, although no significant difference in CSF urea or urea metabolites. Interestingly, CSF urea was only significantly elevated in LATE participants compared to controls. There were no changes in the urea metabolites, citrulline, ornithine and arginine throughout disease; however, we did observe changes in acetate, creatinine, 4-acetamidobutanoate and 4-aminobutyraldehyde which are indirect modifiers of urea. Overall, our study confirms that elevations in urea do occur in HD, albeit later in disease and that these changes may reflect more central impairments to cellular energy metabolism yet to be explored.
Institute:Vanderbilt University
Department:Chemistry
Laboratory:Center for Innovative Technology
Last Name:CODREANU
First Name:SIMONA
Address:1234 STEVENSON CENTER LANE
Email:SIMONA.CODREANU@VANDERBILT.EDU
Phone:6158758422

Subject:

Subject ID:SU002531
Subject Type:Human
Subject Species:Homo sapiens
Taxonomy ID:9606
Gender:Male and female

Factors:

Subject type: Human; Subject species: Homo sapiens (Factor headings shown in green)

mb_sample_id local_sample_id Genotype sex age
SA244189SC_20201109_HILICp_FMS_CSF_E04_C_1_1CONTROL f 47
SA244190SC_20201109_HILICp_FMS_CSF_E11_C_1_2CONTROL f 47
SA244191SC_20201109_HILICp_FMS_CSF_G04_C_1_1CONTROL f 53
SA244192SC_20201109_HILICp_FMS_CSF_G06_C_1_1CONTROL f 53
SA244193SC_20201109_HILICp_FMS_CSF_F01_C_1_2CONTROL f 53
SA244194SC_20201109_HILICp_FMS_CSF_G07_C_1_2CONTROL f 54
SA244195SC_20201109_HILICp_FMS_CSF_D10_C_1_1CONTROL f 58
SA244196SC_20201109_HILICp_FMS_CSF_E12_C_1_2CONTROL f 59
SA244197SC_20201109_HILICp_FMS_CSF_G09_C_1_2CONTROL f 61
SA244198SC_20201109_HILICp_FMS_CSF_G11_C_1_1CONTROL f 61
SA244199SC_20201109_HILICp_FMS_CSF_D01_C_1_1CONTROL m 28
SA244200SC_20201109_HILICp_FMS_CSF_D08_C_1_2CONTROL m 28
SA244201SC_20201109_HILICp_FMS_CSF_C07_C_1_1CONTROL m 32
SA244202SC_20201109_HILICp_FMS_CSF_D09_C_1_2CONTROL m 32
SA244203SC_20201109_HILICp_FMS_CSF_F04_C_1_1CONTROL m 35
SA244204SC_20201109_HILICp_FMS_CSF_F05_C_1_2CONTROL m 36
SA244205SC_20201109_HILICp_FMS_CSF_D06_C_1_2CONTROL m 44
SA244206SC_20201109_HILICp_FMS_CSF_D02_C_1_1CONTROL m 44
SA244207SC_20201109_HILICp_FMS_CSF_F12_C_1_2CONTROL m 51
SA244208SC_20201109_HILICp_FMS_CSF_F06_C_1_1CONTROL m 51
SA244209SC_20201109_HILICp_FMS_CSF_F10_C_1_1CONTROL m 54
SA244210SC_20201109_HILICp_FMS_CSF_G03_C_1_2CONTROL m 54
SA244211SC_20201109_HILICp_FMS_CSF_G05_C_1_2CONTROL m 57
SA244212SC_20201109_HILICp_FMS_CSF_G01_C_1_1CONTROL m 57
SA244213SC_20201109_HILICp_FMS_CSF_F07_HD_3EARLY MANIFEST f 41
SA244214SC_20201109_HILICp_FMS_CSF_H01_HD_3EARLY MANIFEST f 47
SA244215SC_20201109_HILICp_FMS_CSF_B10_HD_3EARLY MANIFEST f 48
SA244216SC_20201109_HILICp_FMS_CSF_G12_HD_3EARLY MANIFEST f 50
SA244217SC_20201109_HILICp_FMS_CSF_F03_HD_3EARLY MANIFEST f 52
SA244218SC_20201109_HILICp_FMS_CSF_A02_HD_3EARLY MANIFEST f 57
SA244219SC_20201109_HILICp_FMS_CSF_G02_HD_3EARLY MANIFEST f 59
SA244220SC_20201109_HILICp_FMS_CSF_F09_HD_3EARLY MANIFEST f 59
SA244221SC_20201109_HILICp_FMS_CSF_H04_HD_3EARLY MANIFEST f 60
SA244222SC_20201109_HILICp_FMS_CSF_A07_HD_3EARLY MANIFEST m 35
SA244223SC_20201109_HILICp_FMS_CSF_C04_HD_3EARLY MANIFEST m 39
SA244224SC_20201109_HILICp_FMS_CSF_D05_HD_3EARLY MANIFEST m 41
SA244225SC_20201109_HILICp_FMS_CSF_G08_HD_3EARLY MANIFEST m 46
SA244226SC_20201109_HILICp_FMS_CSF_A05_HD_3EARLY MANIFEST m 49
SA244227SC_20201109_HILICp_FMS_CSF_A08_HD_3EARLY MANIFEST m 56
SA244228SC_20201109_HILICp_FMS_CSF_C09_HD_3EARLY MANIFEST m 59
SA244229SC_20201109_HILICp_FMS_CSF_A01_HD_4LATE MANIFEST f 38
SA244230SC_20201109_HILICp_FMS_CSF_C02_HD_4LATE MANIFEST f 47
SA244231SC_20201109_HILICp_FMS_CSF_C06_HD_4LATE MANIFEST f 55
SA244232SC_20201109_HILICp_FMS_CSF_C03_HD_4LATE MANIFEST f 57
SA244233SC_20201109_HILICp_FMS_CSF_B01_HD_4LATE MANIFEST f 58
SA244234SC_20201109_HILICp_FMS_CSF_B11_HD_4LATE MANIFEST f 65
SA244235SC_20201109_HILICp_FMS_CSF_E09_HD_4LATE MANIFEST f 72
SA244236SC_20201109_HILICp_FMS_CSF_A10_HD_4LATE MANIFEST m 46
SA244237SC_20201109_HILICp_FMS_CSF_D04_HD_4LATE MANIFEST m 47
SA244238SC_20201109_HILICp_FMS_CSF_D03_HD_4LATE MANIFEST m 51
SA244239SC_20201109_HILICp_FMS_CSF_A06_HD_4LATE MANIFEST m 58
SA244240SC_20201109_HILICp_FMS_CSF_F08_HD_4LATE MANIFEST m 60
SA244241SC_20201109_HILICp_FMS_CSF_A11_HD_4LATE MANIFEST m 60
SA244242SC_20201109_HILICp_FMS_CSF_E07_HD_4LATE MANIFEST m 63
SA244243SC_20201109_HILICp_FMS_CSF_A09_HD_4LATE MANIFEST m 66
SA244244SC_20201109_HILICp_FMS_CSF_D07_HD_4LATE MANIFEST m 69
SA244245SC_20201109_HILICp_FMS_CSF_H03_HD_2_2PRE-MANIFEST f 26
SA244246SC_20201109_HILICp_FMS_CSF_G10_HD_2_1PRE-MANIFEST f 26
SA244247SC_20201109_HILICp_FMS_CSF_B09_HD_2_2PRE-MANIFEST f 30
SA244248SC_20201109_HILICp_FMS_CSF_B03_HD_2_1PRE-MANIFEST f 30
SA244249SC_20201109_HILICp_FMS_CSF_C01_HD_2_2PRE-MANIFEST f 33
SA244250SC_20201109_HILICp_FMS_CSF_C05_HD_2_1PRE-MANIFEST f 33
SA244251SC_20201109_HILICp_FMS_CSF_B04_HD_2_1PRE-MANIFEST f 33
SA244252SC_20201109_HILICp_FMS_CSF_C08_HD_2_2PRE-MANIFEST f 33
SA244253SC_20201109_HILICp_FMS_CSF_B02_HD_2_1PRE-MANIFEST f 36
SA244254SC_20201109_HILICp_FMS_CSF_B08_HD_2_2PRE-MANIFEST f 36
SA244255SC_20201109_HILICp_FMS_CSF_H02_HD_2_1PRE-MANIFEST f 40
SA244256SC_20201109_HILICp_FMS_CSF_C12_HD_2_2PRE-MANIFEST f 40
SA244257SC_20201109_HILICp_FMS_CSF_F11_HD_2_1PRE-MANIFEST f 42
SA244258SC_20201109_HILICp_FMS_CSF_F02_HD_2_2PRE-MANIFEST f 42
SA244259SC_20201109_HILICp_FMS_CSF_E03_HD_2_1PRE-MANIFEST f 43
SA244260SC_20201109_HILICp_FMS_CSF_E10_HD_2_2PRE-MANIFEST f 43
SA244261SC_20201109_HILICp_FMS_CSF_B05_HD_2_1PRE-MANIFEST m 29
SA244262SC_20201109_HILICp_FMS_CSF_B06_HD_2_2PRE-MANIFEST m 29
SA244263SC_20201109_HILICp_FMS_CSF_E06_HD_2_2PRE-MANIFEST m 30
SA244264SC_20201109_HILICp_FMS_CSF_E01_HD_2_1PRE-MANIFEST m 30
SA244265SC_20201109_HILICp_FMS_CSF_E08_HD_2_1PRE-MANIFEST m 31
SA244266SC_20201109_HILICp_FMS_CSF_A04_HD_2_2PRE-MANIFEST m 31
SA244267SC_20201109_HILICp_FMS_CSF_B12_HD_2_2PRE-MANIFEST m 35
SA244268SC_20201109_HILICp_FMS_CSF_B07_HD_2_1PRE-MANIFEST m 35
SA244269SC_20201109_HILICp_FMS_CSF_C11_HD_2_1PRE-MANIFEST m 36
SA244270SC_20201109_HILICp_FMS_CSF_C10_HD_2_2PRE-MANIFEST m 37
SA244271SC_20201109_HILICp_FMS_CSF_D12_HD_2_2PRE-MANIFEST m 42
SA244272SC_20201109_HILICp_FMS_CSF_D11_HD_2_1PRE-MANIFEST m 42
SA244273SC_20201109_HILICp_FMS_CSF_A03_HD_2_1PRE-MANIFEST m 48
SA244274SC_20201109_HILICp_FMS_CSF_E02_HD_2_1PRE-MANIFEST m 48
SA244275SC_20201109_HILICp_FMS_CSF_A12_HD_2_2PRE-MANIFEST m 48
SA244276SC_20201109_HILICp_FMS_CSF_E05_HD_2_2PRE-MANIFEST m 48
Showing results 1 to 88 of 88

Collection:

Collection ID:CO002524
Collection Summary:CSF samples were collected from 60 participants as part of the CHDI HD-Clarity study. There were 16 PRE, 16 MAN, 16 LATE HD participants and 12 control participants. Disease stage was determined using the diagnostic confidence level (DCL), length of CAG expansion and burden of pathology calculated from (CAG expansion – 35.5) x Age. Control participants were individuals without a known history of Huntington Disease (HD). All HD participants have a CAG expansion of > 40. PRE participants were not motor manifest as indicated by a DCL of <4 and a burden of pathology of > 250. MAN participants had a DCL =4 and a total functional capacity (TFC) between 7-13. The LATE group had all the above criteria for MAN and a TFC score between 0-6. Repeat CSF and blood samples collected 4-8 weeks after a baseline (BL) visit are provided for all control and PRE participants. Participants’ age and gender are reported here. Three participants (2 PRE, 1 MAN) were taking supplemental vitamins; however, their metal levels were similar to those in their corresponding participant group and thus, the data from these participants are included. Basic demographics like age and gender were reported previously in addition to participants' scores on a battery of cognitive, behavioral and motor assessments including the symbol digit modality test (SDMT), Stroop Word Reading (SWR), total functional capacity (TFC), total motor score (TMS) and the recently developed cUHDRS.
Collection Protocol Filename:Sample_Collection.pdf
Sample Type:CSF
Storage Conditions:-80℃

Treatment:

Treatment ID:TR002543
Treatment Summary:No treatment

Sample Preparation:

Sampleprep ID:SP002537
Sampleprep Summary:CSF samples collected were flash frozen and stored at -80°C until analyzed via Liquid ChromatographyHigh Resolution Mass Spectrometry (LC-HRMS and LC-HRMS/MS)-based metabolomics in the Vanderbilt Center for Innovative Technology (CIT) using previously described methods (cite). Briefly, equal volumes (100 µL) of previously frozen CSF was diluted with 100 µL ice-cold lysis buffer (1:1:2, Acetonitrile:MeOH:Ammonium Bicarbonate 0.1M, pH 8.0, LC-MS grade). Addition of isotopically labeled phenylalanine-D8 and biotin-D2 were added to individual samples prior to protein precipitation by addition of 800 µL of ice-cold methanol. Following overnight incubation at -80°C, precipitated proteins were pelleted by centrifugation at 10,000 rpm for 10 min and metabolite extracts were dried down in vacuo and stored at -80°C until reconstitution prior to MS analysis.

Combined analysis:

Analysis ID AN003979
Analysis type MS
Chromatography type HILIC
Chromatography system Thermo Vanquish
Column Waters ACQUITY UPLC BEH HILIC (100 x 2.1mm,1.7um)
MS Type ESI
MS instrument type Orbitrap
MS instrument name Thermo Q Exactive HF hybrid Orbitrap
Ion Mode POSITIVE
Units time_m/z

Chromatography:

Chromatography ID:CH002942
Chromatography Summary:CSF extracts (5uL injection volume) were separated on an ACQUITY UPLC BEH Amide HILIC 1.7μm, 2.1 × 100 mm column (Waters Corporation, Milford, MA) held at 30°C as previously described (cite). Briefly, liquid chromatography was performed at 200 µL min−1 using solvent A (5 mM ammonium formate in 90% water, 10% acetonitrile and 0.1% formic acid) and solvent B (5 mM ammonium formate in 90% acetonitrile, 10% water and 0.1% formic acid) with a gradient length of 30 min.
Methods Filename:Metabolomics_Analyses.pdf
Instrument Name:Thermo Vanquish
Column Name:Waters ACQUITY UPLC BEH HILIC (100 x 2.1mm,1.7um)
Column Temperature:30
Flow Gradient:30 min
Flow Rate:0.20mL/min
Solvent A:90% water, 10% acetonitrile, 5mM Ammonium Formate, 0.1%FA
Solvent B:10% water, 90% acetonitrile, 5mM Ammonium Formate, 0.1%FA
Chromatography Type:HILIC

MS:

MS ID:MS003713
Analysis ID:AN003979
Instrument Name:Thermo Q Exactive HF hybrid Orbitrap
Instrument Type:Orbitrap
MS Type:ESI
MS Comments:Full MS analyses were acquired over the mass-to-charge ratio (m/z) range of 70-1,050 in positive ion mode. Full mass scan was acquired at 120,000 resolution with a scan rate of 3.5 Hz, automatic gain control (AGC) target of 1x106, and maximum ion injection time of 100 ms, and MS/MS spectra were collected at 15,000 resolution, AGC target of 2x105 ions, with a maximum ion injection time of 100 ms
Ion Mode:POSITIVE
Analysis Protocol File:Metabolomics_Analyses.pdf
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