Return to study ST000050 main page
MB Sample ID: SA002172
Local Sample ID: | UCON100836 |
Subject ID: | SU000068 |
Subject Type: | Human |
Subject Species: | Homo sapiens |
Taxonomy ID: | 9606 |
Gender: | 24 female; 16 male |
Species Group: | Human |
Select appropriate tab below to view additional metadata details:
Subject:
Subject ID: | SU000068 |
Subject Type: | Human |
Subject Species: | Homo sapiens |
Taxonomy ID: | 9606 |
Gender: | 24 female; 16 male |
Species Group: | Human |
Factors:
Local Sample ID | MB Sample ID | Factor Level ID | Level Value | Factor Name |
---|---|---|---|---|
UCON100836 | SA002172 | FL000662 | 0 | Acute Kidney Injury |
Collection:
Collection ID: | CO000051 |
Collection Summary: | - |
Sample Type: | Urine |
Treatment:
Treatment ID: | TR000069 |
Sample Preparation:
Sampleprep ID: | SP000064 |
Sampleprep Summary: | Frozen urine study samples were thawed on ice and vortexed for 30 seconds. Each of the 40 urine samples (200 µL) were prepared individually by addition of 25 µL D20 and 25 µL Chenomx Internal Standard (Chenomx ISTD, Edmonton, Alberta, Canada). Phenotypic pools for AKI and no AKI were generated with 60 µL of each urine sample pooled, mixed, divided into 3 aliquots. Additionally, 400 µL from both phenotypic pools were mixed to form a total pooled sample and divided into 3 aliquots. The pooled samples were prepared identically to the individual study samples. 1H NMR spectra of urine samples were acquired on a Bruker Avance 950 MHz NMR spectrometer (located at the David H. Murdock Research Institute at Kannapolis, NC, USA) using a 3 mm cryogenically cooled ATMA inverse probe and ambient temperature of 25℃. A 1D NOESY presaturation pulse sequence (noesypr1d, [recycle delay (RD)-90°-t1-90°-tm-90°-acquire free induction decay (FID) was used for data acquisition. For each sample 64 transients were collected into 65k data points using a spectral width of 14.01 kHz (20.14 ppm), 2 s relaxation delay, 100 ms mixing time, and an acquisition time of 2.324 s per FID. The water resonance was suppressed using resonance irradiation during the relaxation delay and mixing time. NMR spectra were processed using Chenomx NMR Suite 7.51 Professional (Chenomx, Edmonton, Alberta, Canada) software. Spectra were zero filled, and Fourier transformed after exponential multiplication with line broadening factor of 0.5. Phase and baseline of the spectra were manually corrected for each spectrum. Spectra were referenced internally to the DSS signal. The quality of each NMR spectrum was assessed for the level of noise and alignment of identified markers. Spectra were assessed for missing data and underwent quality checks. NMR bins (0.50-9.0 ppm) were made after excluding DSS, water (4.68-4.80 ppm), and Imidazole (7.20-7.28 ppm) using bucket Integration with a 0.04 ppm bucket width. Integrals of each of the bins were normalized to total integral of each of the spectrum. |
Sampleprep Protocol Filename: | RTI_NeonatalAKI_Metabolomics_Procedure.docx |
Analysis:
MB Sample ID: | SA002172 |
Analysis ID: | AN000086 |
Laboratory Name: | RTI |
Analysis Type: | NMR |
Software Version: | Top Spin 3.2 |
Chromatography ID: | CH000055 |
Num Factors: | 3 |
NMR:
NMR ID: | NM000023 |
Analysis ID: | AN000086 |
Instrument Name: | Bruker Avance III |
Instrument Type: | FT-NMR |
NMR Experiment Type: | 1D 1H |
Field Frequency Lock: | Deuterium |
Standard Concentration: | 0.5mM |
Spectrometer Frequency: | 950 MHz |
NMR Probe: | cyrogenically cooled ATMA inverse probe |
NMR Solvent: | D2O |
NMR Tube Size: | 3mm |
Shimming Method: | Gradient |
Pulse Sequence: | NOESYpr1d |
Water Suppression: | yes |
Pulse Width: | 19.9298 |
Receiver Gain: | 4 |
Offset Frequency: | 4468.3 |
Chemical Shift Ref Cpd: | formate |
Temperature: | 25 degrees celsius |
Number Of Scans: | 64 |
Dummy Scans: | 4 |
Acquisition Time: | 1.73 seconds |
Spectral Width: | 19.9298 |
Num Data Points Acquired: | 65536 |
Real Data Points: | 65536 |
Line Broadening: | 0.5 |
Zero Filling: | yes |
Apodization: | Lorentzian |
Baseline Correction Method: | quad |