Coupling Capillary Zone Electrophoresis to a Q Exactive HF Mass Spectrometer for Top-down Proteomics: 580 Proteoform Identifications from Yeast

Abstract: We used reversed-phase liquid chromatography to separate the yeast proteome into 23 fractions. These fractions were then analyzed using capillary zone electrophoresis (CZE) coupled to a Q-Exactive HF mass spectrometer using an electrokinetically pumped sheath flow interface. The parameters of the mass spectrometer were first optimized for top-down proteomics using a mixture of seven model proteins; we observed that intact protein mode with trapping pressure of 0.2 and normalized collision energy of 20% produce… Show more

“…[6] Later, Zhao et al further applied the CZE-MS/MS system for top-down proteomics of Mycobacterium marinum secretome and yeast proteome. [7, 8] Coupling offline RPLC fractionation to CZE-MS/MS identified 580 proteoforms from a yeast lysate. In total, 23 RPLC fractions were analyzed by CZE-MS/MS and up to 180 proteoforms could be identified with single-shot CZE-MS/MS.…”

“…In total, 23 RPLC fractions were analyzed by CZE-MS/MS and up to 180 proteoforms could be identified with single-shot CZE-MS/MS. [8] Li et al developed a CZE-MS system based on the electrokinetically pumped sheath flow interface and applied the system to a complex proteome sample for characterization of large proteins (30–80 kDa), resulting in identification of 30 proteins in the mass range of 30–80 kDa. [9] …”

“…First, the largest sample loading capacity of CZE-MS/MS systems reported in the literature for top-down proteomics is only about 200 nL. [8,10] The low sample loading capacity impedes identification of low abundant proteoforms from complex proteome samples. Second, the reported separation window of CZE-MS/MS systems for top-down proteomics is roughly 30 min.…”

“…Second, the reported separation window of CZE-MS/MS systems for top-down proteomics is roughly 30 min. [8,10] The narrow separation window limits the number of MS/MS spectra acquired during one experiment, which restricts the number of proteoform identifications (IDs) from CZE-MS/MS. Capillary isoelectric focusing (cIEF)-MS is a promising technique for large-scale top-down proteomics due to its large sample loading capacity and high resolution for separation of intact proteins.…”

“…Zhao et al performed top-down proteomics of a yeast lysate using dynamic pH junction based CZE-MS/MS. [8] They used 5 mM ammonium bicarbonate (pH 8) as the sample buffer and 5% (v/v) acetic acid (pH 2.4) as the BGE. 100–240 nL of the sample was injected for CZE-MS/MS analysis.…”

Single-Shot Top-Down Proteomics with Capillary Zone Electrophoresis-Electrospray Ionization-Tandem Mass Spectrometry for Identification of Nearly 600 Escherichia coli Proteoforms

“…[6] Later, Zhao et al further applied the CZE-MS/MS system for top-down proteomics of Mycobacterium marinum secretome and yeast proteome. [7, 8] Coupling offline RPLC fractionation to CZE-MS/MS identified 580 proteoforms from a yeast lysate. In total, 23 RPLC fractions were analyzed by CZE-MS/MS and up to 180 proteoforms could be identified with single-shot CZE-MS/MS.…”

“…In total, 23 RPLC fractions were analyzed by CZE-MS/MS and up to 180 proteoforms could be identified with single-shot CZE-MS/MS. [8] Li et al developed a CZE-MS system based on the electrokinetically pumped sheath flow interface and applied the system to a complex proteome sample for characterization of large proteins (30–80 kDa), resulting in identification of 30 proteins in the mass range of 30–80 kDa. [9] …”

“…First, the largest sample loading capacity of CZE-MS/MS systems reported in the literature for top-down proteomics is only about 200 nL. [8,10] The low sample loading capacity impedes identification of low abundant proteoforms from complex proteome samples. Second, the reported separation window of CZE-MS/MS systems for top-down proteomics is roughly 30 min.…”

“…Second, the reported separation window of CZE-MS/MS systems for top-down proteomics is roughly 30 min. [8,10] The narrow separation window limits the number of MS/MS spectra acquired during one experiment, which restricts the number of proteoform identifications (IDs) from CZE-MS/MS. Capillary isoelectric focusing (cIEF)-MS is a promising technique for large-scale top-down proteomics due to its large sample loading capacity and high resolution for separation of intact proteins.…”

“…Zhao et al performed top-down proteomics of a yeast lysate using dynamic pH junction based CZE-MS/MS. [8] They used 5 mM ammonium bicarbonate (pH 8) as the sample buffer and 5% (v/v) acetic acid (pH 2.4) as the BGE. 100–240 nL of the sample was injected for CZE-MS/MS analysis.…”

Single-Shot Top-Down Proteomics with Capillary Zone Electrophoresis-Electrospray Ionization-Tandem Mass Spectrometry for Identification of Nearly 600 Escherichia coli Proteoforms

Capillary Zone Electrophoresis–Mass Spectrometry for Top‐Down Proteomics: Technological Development and Biological Applications

Multidimensional separations in top–down proteomics