Native ambient mass spectrometry of membrane proteins directly from bacterial colonies †

Yuying Du; Helen J. Cooper

doi:10.1039/d4cc03881a

Native ambient mass spectrometry of membrane proteins directly from bacterial colonies †

Yuying Du, Helen J. Cooper^*

^*Corresponding author for this work

Biosciences

Research output: Contribution to journal › Letter › peer-review

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Abstract

Native ambient mass spectrometry (NAMS) enables analysis of protein structure directly from biological substrates by use of liquid junction sampling techniques together with sampling solvents which mimic the proteins’ natural environment. Here, we demonstrate detection of membrane and membrane-associated proteins directly from E. coli by combining liquid extraction surface analysis (LESA) with a straightforward washing protocol, which attenuates soluble proteins and enables detection of membrane proteins.

Original language	English
Journal	Chemical Communications
Early online date	5 Feb 2025
DOIs	https://doi.org/10.1039/d4cc03881a
Publication status	E-pub ahead of print - 5 Feb 2025

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10.1039/d4cc03881aLicence: Creative Commons: Attribution (CC BY)

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Licence for VOR version of this article starting on Feb 05, 2025: https://creativecommons.org/licenses/by/3.0/
Final published version, 677 KBLicence: Creative Commons: Attribution (CC BY)

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title = "Native ambient mass spectrometry of membrane proteins directly from bacterial colonies †",

abstract = "Native ambient mass spectrometry (NAMS) enables analysis of protein structure directly from biological substrates by use of liquid junction sampling techniques together with sampling solvents which mimic the proteins{\textquoteright} natural environment. Here, we demonstrate detection of membrane and membrane-associated proteins directly from E. coli by combining liquid extraction surface analysis (LESA) with a straightforward washing protocol, which attenuates soluble proteins and enables detection of membrane proteins.",

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AU - Du, Yuying

AU - Cooper, Helen J.

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N2 - Native ambient mass spectrometry (NAMS) enables analysis of protein structure directly from biological substrates by use of liquid junction sampling techniques together with sampling solvents which mimic the proteins’ natural environment. Here, we demonstrate detection of membrane and membrane-associated proteins directly from E. coli by combining liquid extraction surface analysis (LESA) with a straightforward washing protocol, which attenuates soluble proteins and enables detection of membrane proteins.

AB - Native ambient mass spectrometry (NAMS) enables analysis of protein structure directly from biological substrates by use of liquid junction sampling techniques together with sampling solvents which mimic the proteins’ natural environment. Here, we demonstrate detection of membrane and membrane-associated proteins directly from E. coli by combining liquid extraction surface analysis (LESA) with a straightforward washing protocol, which attenuates soluble proteins and enables detection of membrane proteins.

U2 - 10.1039/d4cc03881a

DO - 10.1039/d4cc03881a

M3 - Letter

SN - 1359-7345

JO - Chemical Communications

JF - Chemical Communications

ER -

Native ambient mass spectrometry of membrane proteins directly from bacterial colonies †

Abstract

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