Summary of Study ST002890
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 PR001803. The data can be accessed directly via it's Project DOI: 10.21228/M8NQ7P 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.
| Study ID | ST002890 |
| Study Title | Characterization of the in vivo deuteration of native phospholipids by mass spectrometry yields guidelines for their regiospecific customization |
| Study Summary | Customization of deuterated biomolecules is vital for many advanced biological experiments, including neutron scattering. However, because it is challenging to control the proportion and regiospecificity of deuterium incorporation in live systems, often only two or three synthetic lipids are mixed together to form simplistic model membranes. This limits the applicability and biological accuracy of the results generated with these synthetic membranes. Despite some limited prior examination of deuterating E. coli lipids in vivo, this approach has not been widely implemented. Here, an extensive mass spectrometry-based profiling of E. coli phospholipid deuteration states with several different growth media was performed and a computational method to describe deuterium distributions with a one-number summary is introduced. The deuteration states of thirty-six lipid species were quantitatively profiled in fifteen different growth conditions and tandem mass spectrometry was used to reveal deuterium localization. Regressions were employed to enable the prediction of lipid deuteration for untested conditions. Small-angle neutron scattering was performed on select deuterated lipid samples, which validated the deuteration states calculated from the mass spectral data. Based on these experiments, guidelines for the design of specifically deuterated phospholipids are described. This unlocks even greater capabilities from neutron-based techniques, enabling experiments that were formerly impossible. |
| Institute | University of Tennessee |
| Department | Genome Science and Technology (Bredesen Center) |
| Last Name | Matthew |
| First Name | Keller |
| Address | The Bredesen Center for Interdisciplinary Research and Graduate Education 444 Greve Hall, 821 Volunteer Blvd. Knoxville, TN 37996-3394 |
| qrh579@vols.utk.edu | |
| Phone | 18659747999 |
| Submit Date | 2023-09-26 |
| Raw Data Available | Yes |
| Raw Data File Type(s) | mzML |
| Analysis Type Detail | LC-MS |
| Release Date | 2023-10-12 |
| Release Version | 1 |
Select appropriate tab below to view additional metadata details:
Project:
| Project ID: | PR001803 |
| Project DOI: | doi: 10.21228/M8NQ7P |
| Project Title: | Characterization of the in vivo deuteration of native phospholipids by mass spectrometry yields guidelines for their regiospecific customization |
| Project Summary: | Customization of deuterated biomolecules is vital for many advanced biological experiments, including neutron scattering. However, because it is challenging to control the proportion and regiospecificity of deuterium incorporation in live systems, often only two or three synthetic lipids are mixed together to form simplistic model membranes. This limits the applicability and biological accuracy of the results generated with these synthetic membranes. Despite some limited prior examination of deuterating E. coli lipids in vivo, this approach has not been widely implemented. Here, an extensive mass spectrometry-based profiling of E. coli phospholipid deuteration states with several different growth media was performed and a computational method to describe deuterium distributions with a one-number summary is introduced. The deuteration states of thirty-six lipid species were quantitatively profiled in fifteen different growth conditions and tandem mass spectrometry was used to reveal deuterium localization. Regressions were employed to enable the prediction of lipid deuteration for untested conditions. Small-angle neutron scattering was performed on select deuterated lipid samples, which validated the deuteration states calculated from the mass spectral data. Based on these experiments, guidelines for the design of specifically deuterated phospholipids are described. This unlocks even greater capabilities from neutron-based techniques, enabling experiments that were formerly impossible. |
| Institute: | University of Tennessee |
| Department: | Genome Science and Technology (Bredesen Center) |
| Last Name: | Matthew |
| First Name: | Keller |
| Address: | The Bredesen Center for Interdisciplinary Research and Graduate Education 444 Greve Hall, 821 Volunteer Blvd |
| Email: | qrh579@vols.utk.edu |
| Phone: | 18659747999 |
| Publications: | In review at Analytical Chemistry |
| Contributors: | Qiu Zhang, Shuo Qian, Brian Sanders, Hugh O'Neill, Robert Hettich |
Subject:
| Subject ID: | SU003003 |
| Subject Type: | Bacteria |
| Subject Species: | Escherichia coli |
| Genotype Strain: | BL21(DE3) |
Factors:
Subject type: Bacteria; Subject species: Escherichia coli (Factor headings shown in green)
| mb_sample_id | local_sample_id | Carbon source | Percent D2O | MS ionization mode |
|---|---|---|---|---|
| SA315384 | H-Glu/25_2-neg | 50/50 H/D-Glycerol | 0 | negative |
| SA315385 | H-Glu/25_3-neg | 50/50 H/D-Glycerol | 0 | negative |
| SA315386 | H-Glu/25_1-neg | 50/50 H/D-Glycerol | 0 | negative |
| SA315387 | H-Glu/25_3-pos | 50/50 H/D-Glycerol | 0 | positive |
| SA315388 | H-Glu/25_2-pos | 50/50 H/D-Glycerol | 0 | positive |
| SA315389 | H-Glu/25_1-pos | 50/50 H/D-Glycerol | 0 | positive |
| SA315390 | H-Glu/75_1-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315391 | H-Glu/75_repeat_2-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315392 | H-Glu/75_repeat_1-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315393 | H-Glu/75_3-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315394 | H-Glu/75_2-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315395 | H-Glu/75_repeat_3-neg | 50/50 H/D-Glycerol | 100 | negative |
| SA315396 | H-Glu/75_3-pos | 50/50 H/D-Glycerol | 100 | positive |
| SA315397 | H-Glu/75_1-pos | 50/50 H/D-Glycerol | 100 | positive |
| SA315398 | H-Glu/75_2-pos | 50/50 H/D-Glycerol | 100 | positive |
| SA315399 | D-Glu/100-neg_tech-rep1 | D-Glucose | 0 | negative |
| SA315400 | D-Glu/100-neg_tech-rep2 | D-Glucose | 0 | negative |
| SA315401 | D-Glu/100-pos | D-Glucose | 0 | positive |
| SA315402 | 50D-Gly/100_2-neg | D-Glucose | 100 | negative |
| SA315403 | 50D-Gly/100_3-neg | D-Glucose | 100 | negative |
| SA315404 | 50D-Gly/100_1-neg | D-Glucose | 100 | negative |
| SA315405 | 50D-Gly/100_1-pos | D-Glucose | 100 | positive |
| SA315406 | 50D-Gly/100_2-pos | D-Glucose | 100 | positive |
| SA315407 | 50D-Gly/100_3-pos | D-Glucose | 100 | positive |
| SA315408 | H-Glu/50_1-neg | D-Glycerol | 0 | negative |
| SA315409 | H-Glu/50_2-neg | D-Glycerol | 0 | negative |
| SA315410 | H-Glu/50_3-neg | D-Glycerol | 0 | negative |
| SA315411 | H-Glu/50_2-pos | D-Glycerol | 0 | positive |
| SA315412 | H-Glu/50_3-pos | D-Glycerol | 0 | positive |
| SA315413 | H-Glu/50_1-pos | D-Glycerol | 0 | positive |
| SA315414 | H-Glu/100-neg_tech-rep2 | D-Glycerol | 100 | negative |
| SA315415 | H-Glu/100-neg_tech-rep1 | D-Glycerol | 100 | negative |
| SA315416 | H-Glu/100-pos | D-Glycerol | 100 | positive |
| SA315417 | 50D-Gly/0_1-neg | H-Glucose | 100 | negative |
| SA315418 | 50D-Gly/0_2-neg | H-Glucose | 100 | negative |
| SA315419 | 50D-Gly/0_3-neg | H-Glucose | 100 | negative |
| SA315420 | 50D-Gly/0_2-pos | H-Glucose | 100 | positive |
| SA315421 | 50D-Gly/0_1-pos | H-Glucose | 100 | positive |
| SA315422 | 50D-Gly/0_3-pos | H-Glucose | 100 | positive |
| SA315423 | D-Glu/0_3-neg | H-Glucose | 25 | negative |
| SA315424 | D-Glu/0_2-neg | H-Glucose | 25 | negative |
| SA315425 | D-Glu/0_1-neg | H-Glucose | 25 | negative |
| SA315426 | D-Glu/0_2-pos | H-Glucose | 25 | positive |
| SA315427 | D-Glu/0_1-pos | H-Glucose | 25 | positive |
| SA315428 | D-Glu/0_3-pos | H-Glucose | 25 | positive |
| SA315429 | D-Gly/0_2-neg | H-Glucose | 50 | negative |
| SA315430 | D-Gly/0_1-neg | H-Glucose | 50 | negative |
| SA315431 | D-Gly/0_3-neg | H-Glucose | 50 | negative |
| SA315432 | D-Gly/0_3-pos | H-Glucose | 50 | positive |
| SA315433 | D-Gly/0_2-pos | H-Glucose | 50 | positive |
| SA315434 | D-Gly/0_1-pos | H-Glucose | 50 | positive |
| SA315435 | D-Gly/100_2-neg | H-Glucose | 75 | negative |
| SA315436 | D-Gly/100_3-neg | H-Glucose | 75 | negative |
| SA315437 | D-Gly/100_1-neg | H-Glucose | 75 | negative |
| SA315438 | D-Gly/100_3-pos | H-Glucose | 75 | positive |
| SA315439 | D-Gly/100_1-pos | H-Glucose | 75 | positive |
| SA315440 | D-Gly/100_2-pos | H-Glucose | 75 | positive |
| SA315441 | H-Gly/0-neg_tech-rep2 | H-Glycerol | 0 | negative |
| SA315442 | H-Gly/0-neg_tech-rep1 | H-Glycerol | 0 | negative |
| SA315443 | H-Gly/0-pos | H-Glycerol | 0 | positive |
| SA315444 | H-Gly/100_1-neg | H-Glycerol | 100 | negative |
| SA315445 | H-Gly/100_2-neg | H-Glycerol | 100 | negative |
| SA315446 | H-Gly/100_3-neg | H-Glycerol | 100 | negative |
| SA315447 | H-Gly/100_3-pos | H-Glycerol | 100 | positive |
| SA315448 | H-Gly/100_2-pos | H-Glycerol | 100 | positive |
| SA315449 | H-Gly/100_1-pos | H-Glycerol | 100 | positive |
| SA315450 | H-Gly/25-neg_tech-rep2 | H-Glycerol | 25 | negative |
| SA315451 | H-Gly/25-neg_tech-rep1 | H-Glycerol | 25 | negative |
| SA315452 | H-Gly/25-pos | H-Glycerol | 25 | positive |
| SA315453 | H-Gly/50-neg_tech-rep1 | H-Glycerol | 50 | negative |
| SA315454 | H-Gly/50-neg_tech-rep2 | H-Glycerol | 50 | negative |
| SA315455 | H-Gly/50-pos | H-Glycerol | 50 | positive |
| SA315456 | H-Gly/75-neg_tech-rep2 | H-Glycerol | 75 | negative |
| SA315457 | H-Gly/75-neg_tech-rep1 | H-Glycerol | 75 | negative |
| SA315458 | H-Gly/75-pos | H-Glycerol | 75 | positive |
| Showing results 1 to 75 of 75 |
Collection:
| Collection ID: | CO002996 |
| Collection Summary: | Lipids were extracted from E coli cell pellets following the Matyash protocol with slight variations described in the manuscript supplemental. Cell lysis was performed with bead beating or ultrasonication. Extraction solvents were in the ratio 10:3:25 MTBE:methanol:water. See publication for more detail. |
| Collection Protocol Filename: | Deuterated_Lipids_Methods_Summary.pdf |
| Sample Type: | Bacterial cells |
Treatment:
| Treatment ID: | TR003012 |
| Treatment Summary: | E. coli was grown in Enfors minimal media (deuterated or otherwise) with different carbon sources including glycerol, glucose, D-glycerol, and D-glucose. |
| Cell Media: | Enfors minimal media |
| Cell Harvesting: | 30 mL culture collected by centrifugation at 4k x g |
Sample Preparation:
| Sampleprep ID: | SP003009 |
| Sampleprep Summary: | Lipids were extracted from E coli cell pellets following the Matyash protocol with slight variations described in the manuscript supplemental. Cell lysis was performed with bead beating or ultrasonication. Extraction solvents were in the ratio 10:3:25 MTBE:methanol:water. See publication for more detail. |
| Sampleprep Protocol Filename: | Deuterated_Lipids_Methods_Summary.pdf |
| Extraction Method: | Matyash (MTBE) varient |
| Sample Resuspension: | 8:23:69 butanol:isopropanol:water |
Combined analysis:
| Analysis ID | AN004748 | AN004749 |
|---|---|---|
| Analysis type | MS | MS |
| Chromatography type | Reversed phase | Reversed phase |
| Chromatography system | Thermo Dionex Ultimate 3000 RS | Thermo Dionex Ultimate 3000 RS |
| Column | In-house packed nano column (ID 100 μm, Kinetex 1.7 μm C18 (100 Å) [Phenomenex], 12-15 cm. | In-house packed nano column (ID 100 μm, Kinetex 1.7 μm C18 (100 Å) [Phenomenex], 12-15 cm. |
| MS Type | ESI | ESI |
| MS instrument type | LTQ-FT | LTQ-FT |
| MS instrument name | Thermo Velos Pro Orbitrap | Thermo Velos Pro Orbitrap |
| Ion Mode | NEGATIVE | POSITIVE |
| Units | Presence/Absence | Presence/Absence |
Chromatography:
| Chromatography ID: | CH003581 |
| Chromatography Summary: | Because the columns were packed in-house, there is some variation in the total length (see column description below). |
| Methods Filename: | Deuterated_Lipids_Methods_Summary.pdf |
| Instrument Name: | Thermo Dionex Ultimate 3000 RS |
| Column Name: | In-house packed nano column (ID 100 μm, Kinetex 1.7 μm C18 (100 Å) [Phenomenex], 12-15 cm. |
| Column Temperature: | room temp |
| Flow Gradient: | Solvent Gradient: Time (min) 0 1 2.5 7.5 13.5 48.5 58.5 75.5 77.5 87 Solvent A (%) 99 99 70 65 45 30 1 1 99 99 Solvent B (%) 1 1 30 45 55 70 99 99 1 1 |
| Flow Rate: | Split flow nano-chromatography. The actual flow rate at the column is dependent on a variety of factors and an accurate measurement of the flow rate is impractical. The flow rate at the macro pumps were set at either 0.05 or 0.1 mL/min depending on the waste line's backpressure. |
| Solvent A: | 60% acetonitrile/40% water; ~0.4g/L ammonium acetate |
| Solvent B: | 90% sopropanol/10% acetonitrile; ~0.4g/L ammonium acetate |
| Chromatography Type: | Reversed phase |
MS:
| MS ID: | MS004494 |
| Analysis ID: | AN004748 |
| Instrument Name: | Thermo Velos Pro Orbitrap |
| Instrument Type: | LTQ-FT |
| MS Type: | ESI |
| MS Comments: | Top 10 DDA acquisition: Oribitrap Full-Scan at 30k resolving power from 150-2000 m/z. Data-dependent collisional-induced dissociation (CID) fragmentation scans performed with the LTQ ion trap at 30 normalized collision energy with normal scan rate. |
| Ion Mode: | NEGATIVE |
| Analysis Protocol File: | Deuterated_Lipids_Methods_Summary.pdf |
| MS ID: | MS004495 |
| Analysis ID: | AN004749 |
| Instrument Name: | Thermo Velos Pro Orbitrap |
| Instrument Type: | LTQ-FT |
| MS Type: | ESI |
| MS Comments: | Top 10 DDA acquisition: Oribitrap Full-Scan at 30k resolving power from 150-2000 m/z. Data-dependent collisional-induced dissociation (CID) fragmentation scans performed with the LTQ ion trap at 30 normalized collision energy with normal scan rate. |
| Ion Mode: | POSITIVE |
| Analysis Protocol File: | Deuterated_Lipids_Methods_Summary.pdf |
