Analysis of Mammalian Cell Proliferation and Macromolecule Synthesis Using Deuterated Water and Gas Chromatography-Mass Spectrometry

Foletta, Victoria C.; Palmieri, Michelle; Kloehn, Joachim; Mason, Shaun; Previs, Stephen F.; McConville, Malcolm J.; Sieber, Oliver M.; Bruce, Clinton R.; Kowalski, Greg M.

doi:10.3390/metabo6040034

Cited by 23 publications

(33 citation statements)

References 59 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The DNA pellet was left to dry for 15 min, then resuspended in H 2 O (200 μL) and was incubated at 55 °C for 10 min followed by vortex mixing. The resuspended DNA samples were hydrolyzed and dephosphorylated by the addition of S1 nuclease and potato acid phosphatase as previously described [17]. After hydrolysis, the deoxyribose moiety was derivatized in a two-step reaction as we have previously detailed [17].…”

Section: Methodsmentioning

confidence: 99%

“…The resuspended DNA samples were hydrolyzed and dephosphorylated by the addition of S1 nuclease and potato acid phosphatase as previously described [17]. After hydrolysis, the deoxyribose moiety was derivatized in a two-step reaction as we have previously detailed [17]. The perfluorotriacetyl derivative of DNA-bound deoxyribose was analyzed by GC–MS in the negative chemical ionization (NCI) mode (Agilent 7890B GC system and an Agilent 5977B MSD) with helium as the carrier and methane as the reagent gas.…”

Section: Methodsmentioning

confidence: 99%

See 1 more Smart Citation

Phosphatidylserine decarboxylase is critical for the maintenance of skeletal muscle mitochondrial integrity and muscle mass

Selathurai

Kowalski

Mason

et al. 2019

Molecular Metabolism

View full text Add to dashboard Cite

Objective Phosphatidylethanolamine (PtdEtn) is a major phospholipid in mammals. It is synthesized via two pathways, the CDP-ethanolamine pathway in the endoplasmic reticulum and the phosphatidylserine (PtdSer) decarboxylase (PSD) pathway in the mitochondria. While the CDP-ethanolamine pathway is considered the major route for PtdEtn synthesis in most mammalian tissues, little is known about the importance of the PSD pathway in vivo, especially in tissues enriched with mitochondria such as skeletal muscle. Therefore, we aimed to examine the role of the mitochondrial PSD pathway in regulating PtdEtn homeostasis in skeletal muscle in vivo . Methods To determine the functional significance of this pathway in skeletal muscle in vivo , an adeno-associated viral vector approach was employed to knockdown PSD expression in skeletal muscle of adult mice. Muscle lipid and metabolite profiling was performed using mass spectrometry. Results PSD knockdown disrupted muscle phospholipid homeostasis leading to an ∼25% reduction in PtdEtn and an ∼45% increase in PtdSer content. This was accompanied by the development of a severe myopathy, evident by a 40% loss in muscle mass as well as extensive myofiber damage as shown by increased DNA synthesis and central nucleation. In addition, PSD knockdown caused marked accumulation of abnormally appearing mitochondria that exhibited severely disrupted inner membrane integrity and reduced OXPHOS protein content. Conclusions The PSD pathway has a significant role in maintaining phospholipid homeostasis in adult skeletal muscle. Moreover, PSD is essential for maintenance of mitochondrial integrity and skeletal muscle mass.

show abstract

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Phosphatidylserine decarboxylase is critical for the maintenance of skeletal muscle mitochondrial integrity and muscle mass

Selathurai

Kowalski

Mason

et al. 2019

Molecular Metabolism

View full text Add to dashboard Cite

show abstract

“…Hexane and aqueous layers were dried at 50°C and 70°C, respectively, under N 2 gas. Selected ion monitoring (SIM) was performed a 159m/z (M 0 ) to 164m/z to obtain the peak areas of both derivatized glycerol triacetate ion and d 5 -glycerol triacetate ion, respectively (Foletta et al, 2016). Glycerol in the samples was quantified using an unlabeled glycerol standard series normalized to the internal standard (d 5 -glycerol).…”

Section: Hydrolysis Of Lipid Fractionsmentioning

confidence: 99%

The assimilation of glycerol into lipid acyl chains and associated carbon backbones of Nannochloropsis salina varies under nitrogen replete and deplete conditions

Poddar

Doomun

Callahan

et al. 2020

Biotech & Bioengineering

View full text Add to dashboard Cite

Mixotrophic cultivation can increase microalgae productivity, yet the associated lipid metabolism remains mostly unknown. Stable isotope labeling was used to track assimilation of glycerol into the triacylglyceride (TAG) and membrane lipids of Nannochloropsis salina. In N-replete media, glycerol uptake and 13 C incorporation into acyl chains were, respectively, 6-fold and 12-fold higher than in N-deplete conditions. In N-replete cultures, 42% of the carbon in the consumed glycerol was assimilated into lipid acyl chains, mostly in membrane lipids rather than TAG. In Ndeplete cultures, only 11% of the limited amount of consumed glycerol was fixed into lipid acyl chains. Labeled lipid-associated glycerol backbones were predominantly 13 C 3 labeled, suggesting that intact glycerol molecules were directly esterified with fatty acids/polar head groups. However, the presence of singly and doubly labeled lipid-bound glycerol species suggested that some glycerol also went through the central carbon metabolism before forming glycerol-3-phosphate destined for lipid esterification. 13 C incorporation was higher in the saturated and monounsaturated than the polyunsaturated acyl chains of TAG, indicating the flux of carbon from glycerol went first to de novo fatty acid synthesis before acyl editing reactions. The results demonstrate that nitrogen availability influences both glycerol consumption and utilization for lipid synthesis in Nannochloropsis, providing novel insights for developing mixotrophic cultivation strategies.

show abstract

“…By adding D2O to the drinking water of mice, previous studies showed the incorporation of deuterium into the total biomass in various mouse organs but could not image and differentiate D-labeled lipids and proteins in situ [5][6][7][8] . Using DO-SRS imaging with macromolecular selectivity, we found that different mouse organs show metabolic preference to either protein or lipid biosynthesis, which reflects their different functions (Supplementary Figure 4A).…”

Section: Visualizing De Novo Lipogenesis and Metabolic Homeostasis Inmentioning

confidence: 99%

“…By applying DO-SRS to living cells and animals, we not only demonstrated its broad utility, high sensitivity, noninvasiveness, subcellular resolution, compatibility with other imaging modality, and suitability for in vivo live imaging in mammals, but also gained new insights on the metabolic basis of several biological processes. respectively [6][7][8] (Figure 1A). As often the rate-limiting step, the synthesis of C-D bondcontaining macromolecules from the precursors is governed by cellular metabolic activities.…”

Section: Introductionmentioning

confidence: 99%

Optical Imaging of Metabolic Dynamics in Animals

Shi

Zheng

Shen

et al. 2018

Preprint

View full text Add to dashboard Cite

Direct visualization of metabolic dynamics in living tissues with high spatial and temporal resolution is essential to understanding many biological processes. Here we introduce a platform that combines deuterium oxide (D2O) probing with stimulated Raman scattering microscopy (DO-SRS) to image in situ metabolic activities. Enzymatic incorporation of D2O-derived deuterium into macromolecules generates carbondeuterium (C-D) bonds, which track biosynthesis in tissues and can be imaged by SRS in situ. Within the broad vibrational spectra of C-D bonds, we discovered lipid-, protein-, and DNA-specific Raman shifts and developed spectral unmixing methods to obtain C-D signals with macromolecular selectivity. DO-SRS enabled us to probe de novo lipogenesis in animals, image protein biosynthesis without tissue bias, and simultaneously visualize lipid and protein metabolism and reveal their different dynamics. DO-SRS, being noninvasive, universally applicable, and cost-effective, can be adapted to a broad range of biological systems to study development, tissue homeostasis, aging, and tumor heterogeneity. Results SRS imaging enables D2O to be a contrast agent for metabolic activitiesWater (H2O), the ubiquitous solvent of life, diffuses freely across cell and organelle membranes and participates in the vast majority of biochemical reactions. As an isotopologue of water, heavy water (D2O) can rapidly equilibrate with total body water in all cells within an organism and label cellular biomolecules with deuterium (D) by forming a variety of X-D bonds through non-enzymatic H/D exchange and enzymatic incorporation ( Figure 1A). The former is spontaneous and reversibly forms oxygen-deuterium (O-D), nitrogen-deuterium (N-D), and sulfur-deuterium (S-D) bonds on existing molecules, whereas the latter depends on enzyme-catalyzed chemical transformation that irreversibly breaks the O-D bond and forms C-D bonds on newly synthesized molecules 5 . Through such transformation, deuterium quickly labels the metabolic precursors, such as non-essential amino acids (NEAAs), acetyl-CoA, and deoxyribose, which are then slowly incorporated into proteins, lipids, and DNA,

show abstract

Analysis of Mammalian Cell Proliferation and Macromolecule Synthesis Using Deuterated Water and Gas Chromatography-Mass Spectrometry

Cited by 23 publications

References 59 publications

Phosphatidylserine decarboxylase is critical for the maintenance of skeletal muscle mitochondrial integrity and muscle mass

Phosphatidylserine decarboxylase is critical for the maintenance of skeletal muscle mitochondrial integrity and muscle mass

The assimilation of glycerol into lipid acyl chains and associated carbon backbones of Nannochloropsis salina varies under nitrogen replete and deplete conditions

Optical Imaging of Metabolic Dynamics in Animals

Contact Info

Product

Resources

About