Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis

Kathrin Rösch; Marcel Kwiatkowski; Hartmut Schlüter; Eva Herker

doi:10.3791/55585

Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis

Standard

Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis. / Rösch, Kathrin; Kwiatkowski, Marcel; Schlüter, Hartmut; Herker, Eva.

In: JOVE-J VIS EXP, No. 122, 17.04.2017.

Research output: SCORING: Contribution to journal › SCORING: Journal article › Research › peer-review

Harvard

Rösch, K, Kwiatkowski, M, Schlüter, H & Herker, E 2017, 'Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis', JOVE-J VIS EXP, no. 122. https://doi.org/10.3791/55585

APA

Rösch, K., Kwiatkowski, M., Schlüter, H., & Herker, E. (2017). Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis. JOVE-J VIS EXP, (122). https://doi.org/10.3791/55585

Vancouver

Rösch K, Kwiatkowski M, Schlüter H, Herker E. Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis. JOVE-J VIS EXP. 2017 Apr 17;(122). https://doi.org/10.3791/55585

Bibtex

@article{914ca53afb7a4fa2bbc413526720b797,

title = "Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis",

abstract = "Lipid droplets are vital to the replication of a variety of different pathogens, most prominently the Hepatitis C Virus (HCV), as the putative site of virion morphogenesis. Quantitative lipid droplet proteome analysis can be used to identify proteins that localize to or are displaced from lipid droplets under conditions such as virus infections. Here, we describe a protocol that has been successfully used to characterize the changes in the lipid droplet proteome following infection with HCV. We use Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC) and thus label the complete proteome of one population of cells with {"}heavy{"} amino acids to quantitate the proteins by mass spectrometry. For lipid droplet isolation, the two cell populations (i.e. HCV-infected/{"}light{"} amino acids and uninfected control/{"}heavy{"} amino acids) are mixed 1:1 and lysed mechanically in hypotonic buffer. After removing the nuclei and cell debris by low speed centrifugation, lipid droplet-associated proteins are enriched by two subsequent ultracentrifugation steps followed by three washing steps in isotonic buffer. The purity of the lipid droplet fractions is analyzed by western blotting with antibodies recognizing different subcellular compartments. Lipid droplet-associated proteins are then separated by SDS-polyacrylamide gel electrophoresis (SDS-PAGE) followed by Coomassie staining. After tryptic digest, the peptides are quantified by liquid chromatography-electrospray ionization-tandem mass spectrometry (LC-ESI-MS/MS). Using this method, we identified proteins recruited to lipid droplets upon HCV infection that might represent pro- or antiviral host factors. Our method can be applied to a variety of different cells and culture conditions, such as infection with pathogens, environmental stress, or drug treatment.",

keywords = "Journal Article",

author = "Kathrin R{\"o}sch and Marcel Kwiatkowski and Hartmut Schl{\"u}ter and Eva Herker",

year = "2017",

month = apr,

day = "17",

doi = "10.3791/55585",

language = "English",

journal = "JOVE-J VIS EXP",

issn = "1940-087X",

publisher = "MYJoVE Corporation",

number = "122",

}

RIS

TY - JOUR

T1 - Lipid Droplet Isolation for Quantitative Mass Spectrometry Analysis

AU - Rösch, Kathrin

AU - Kwiatkowski, Marcel

AU - Schlüter, Hartmut

AU - Herker, Eva

PY - 2017/4/17

Y1 - 2017/4/17

N2 - Lipid droplets are vital to the replication of a variety of different pathogens, most prominently the Hepatitis C Virus (HCV), as the putative site of virion morphogenesis. Quantitative lipid droplet proteome analysis can be used to identify proteins that localize to or are displaced from lipid droplets under conditions such as virus infections. Here, we describe a protocol that has been successfully used to characterize the changes in the lipid droplet proteome following infection with HCV. We use Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC) and thus label the complete proteome of one population of cells with "heavy" amino acids to quantitate the proteins by mass spectrometry. For lipid droplet isolation, the two cell populations (i.e. HCV-infected/"light" amino acids and uninfected control/"heavy" amino acids) are mixed 1:1 and lysed mechanically in hypotonic buffer. After removing the nuclei and cell debris by low speed centrifugation, lipid droplet-associated proteins are enriched by two subsequent ultracentrifugation steps followed by three washing steps in isotonic buffer. The purity of the lipid droplet fractions is analyzed by western blotting with antibodies recognizing different subcellular compartments. Lipid droplet-associated proteins are then separated by SDS-polyacrylamide gel electrophoresis (SDS-PAGE) followed by Coomassie staining. After tryptic digest, the peptides are quantified by liquid chromatography-electrospray ionization-tandem mass spectrometry (LC-ESI-MS/MS). Using this method, we identified proteins recruited to lipid droplets upon HCV infection that might represent pro- or antiviral host factors. Our method can be applied to a variety of different cells and culture conditions, such as infection with pathogens, environmental stress, or drug treatment.

AB - Lipid droplets are vital to the replication of a variety of different pathogens, most prominently the Hepatitis C Virus (HCV), as the putative site of virion morphogenesis. Quantitative lipid droplet proteome analysis can be used to identify proteins that localize to or are displaced from lipid droplets under conditions such as virus infections. Here, we describe a protocol that has been successfully used to characterize the changes in the lipid droplet proteome following infection with HCV. We use Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC) and thus label the complete proteome of one population of cells with "heavy" amino acids to quantitate the proteins by mass spectrometry. For lipid droplet isolation, the two cell populations (i.e. HCV-infected/"light" amino acids and uninfected control/"heavy" amino acids) are mixed 1:1 and lysed mechanically in hypotonic buffer. After removing the nuclei and cell debris by low speed centrifugation, lipid droplet-associated proteins are enriched by two subsequent ultracentrifugation steps followed by three washing steps in isotonic buffer. The purity of the lipid droplet fractions is analyzed by western blotting with antibodies recognizing different subcellular compartments. Lipid droplet-associated proteins are then separated by SDS-polyacrylamide gel electrophoresis (SDS-PAGE) followed by Coomassie staining. After tryptic digest, the peptides are quantified by liquid chromatography-electrospray ionization-tandem mass spectrometry (LC-ESI-MS/MS). Using this method, we identified proteins recruited to lipid droplets upon HCV infection that might represent pro- or antiviral host factors. Our method can be applied to a variety of different cells and culture conditions, such as infection with pathogens, environmental stress, or drug treatment.

KW - Journal Article

U2 - 10.3791/55585

DO - 10.3791/55585

M3 - SCORING: Journal article

C2 - 28448054

JO - JOVE-J VIS EXP

JF - JOVE-J VIS EXP

SN - 1940-087X

IS - 122

ER -