Direct Tandem Mass Spectrometry Reveals Limitations in Protein Profiling Experiments for Plasma Biomarker Discovery

Koomen, John M.; Li, Donghui; Liang, Xiao; Liu, Thomas C.; Coombes, Kevin R.; Abbruzzese, James L.; Kobayashi, Ryûji

doi:10.1021/pr050046x

Cited by 201 publications

(220 citation statements)

References 81 publications

(123 reference statements)

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“…One of these ladders is derived from fibrinogen alpha as shown in Table 2. This ladder is similar to non-phosphorylated endogenous peptide ladder described previously [2,31]. Another ladder of phosphopeptides coming from alpha-2-HS-glycoprotein was also detected.…”

Section: Discussionsupporting

confidence: 84%

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Analysis of human serum phosphopeptidome by a focused database searching strategy

Zhu

Wang

Cheng

et al. 2013

Journal of Proteomics

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Section: Discussionsupporting

confidence: 84%

“…Due to the presence of active exopeptidases in serum, non-phosphorylated endogenous peptide ladders were observed in peptidomic studies [2,31]. In this study, several phosphopeptide ladders were also observed.…”

Section: Discussionmentioning

confidence: 53%

Analysis of human serum phosphopeptidome by a focused database searching strategy

Zhu

Wang

Cheng

et al. 2013

Journal of Proteomics

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“…This has been reported previously and may be due to the presence of degradation products of the most abundant serum proteins. 31,32 Protein A/G depletion did not impact sequence coverage of IgG, likely due to saturation of the column by the abundant immunoglobulins. Similarly, C3 and C8 bead-based fractionation did not significantly change the hydrophobicity distribution of the identified proteins relative to unfractionated serum, nor did fractionation by WCX beads impact the distribution of isoelectric points (Table 4).…”

Section: Lc-ms/ms On a Linear Ion Trap: (3) The Variability Of Peptidmentioning

confidence: 97%

Head-to-Head Comparison of Serum Fractionation Techniques

et al. 2006

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Multiple approaches for simplifying the serum proteome have been described. These techniques are generally developed across different laboratories, samples, mass spectrometry platforms, and analysis tools. Hence, comparing the available schemes is impossible from the existing literature because of confounding variables. We describe a head-to-head comparison of several serum fractionation schemes, including N-linked glycopeptide enrichment, cysteinyl-peptide enrichment, magnetic bead separation (C3, C8, and WCX), size fractionation, protein A/G depletion, and immunoaffinity column depletion of abundant serum proteins. Each technique was compared to results obtained from unfractionated human serum. The results show immunoaffinity subtraction is the most effective means for simplifying the serum proteome while maintaining reasonable sample throughput. The reported dataset is publicly available and provides a standard against which emergent technologies can be compared and evaluated for their contribution to serum-based biomarker discovery.

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Section: Hydrolysis Of Biologically Relevant Peptides In Vivomentioning

confidence: 99%

“…Recently, over 250 peptides up to a mass of 5500 d were identified as derivatives of plasma proteins released by plasmin, thrombin or complement proteases [89]. In almost all cases there were peptide isoforms lacking the predicted C-terminal Arg or Lys residues and it was considered to be evidence of hydrolysis by CPN [89]. Whether this cleavage has physiological significance is unknown as the biological activities of these peptides have not been tested, but it should be taken into consideration when measuring peptide levels as biomarkers.…”

Section: Hydrolysis Of Biologically Relevant Peptides In Vivomentioning

confidence: 99%

Structure and function of human plasma carboxypeptidase N, the anaphylatoxin inactivator

Skidgel

Erdös

2007

International Immunopharmacology

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Human carboxypeptidase N (CPN) was discovered in the early 1960s as a plasma enzyme that inactivates bradykinin and was identified 8 years later as the major "anaphylatoxin inactivator" of blood. CPN plays in important role in protecting the body from excessive buildup of potentially deleterious peptides that normally act as local autocrine or paracrine hormones. This review summarizes the structure, enzymatic properties and function of this important human enzyme, including insights gained by the recent elucidation of the crystal structure of the CPN catalytic subunit and structural modeling of the non-catalytic regulatory 83 kDa subunit. We also discuss its physiological role in cleaving substrates such as kinins, anaphylatoxins, creatine kinase, plasminogen receptors, hemoglobin and stromal cell-derived factor-1α (SDF-1α). HistoryCarboxypeptidases were initially isolated from pancreatic extracts and so were associated with protein and peptide degradation in the digestive tract [1][2][3][4]. However, work beginning in the early 1960's by Erdös and Sloane [5] revealed the presence of a novel carboxypeptidase in the blood that plays a regulatory role by inactivating bradykinin via removal of its C-terminal Arg residue. (Subsequent research some 2 decades later led to the discovery of a second kinin B 1 receptor activated by the carboxypeptidase metabolite that is its endogenous agonist -see below). Initially it was assumed that the enzyme represents a circulating form of pancreatic carboxypeptidase B, but this was disproved by the characterization of its enzymatic properties [5][6][7][8], which was later borne out by biochemical studies, sequence analysis [9][10][11][12][13][14][15] and ultimately X-ray crystallography [16]. To differentiate it from the pancreatic enzyme, it was named carboxypeptidase N (CPN; EC 3.4.17.3) and was the first member of a family of carboxypeptidases now known as the regulatory or CPN/E subfamily of metallocarboxypeptidases [17][18][19]. It has since been re-discovered many times as other substrates were found and so has acquired aliases such as creatine kinase conversion factor, plasma carboxypeptidase B, arginine carboxypeptidase, lysine carboxypeptidase and protaminase [8,17,20,21]. The most notable was the finding by Bokisch and Müller-Eberhard in 1969 -70 [22,23] that the human plasma "anaphylatoxin inactivator" is identical with CPN. This finding explains our interest in the work of Dr. Tony Hugli, who has made many seminal contributions to the understanding of the structure and function of anaphylatoxins [24][25][26][27]. In Send Correspondence and Proofs To: Randal A. Skidgel, PhD, Dept. of Pharmacology (M/C 868), Univ. of Illinois College of Medicine, 835 S. Wolcott, Chicago, IL 60612, Phone: 312-996-9179, FAX: 312-996-1648, EMAIL: E-mail: rskidgel@uic.edu. Publisher's Disclaimer: This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript w...

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Direct Tandem Mass Spectrometry Reveals Limitations in Protein Profiling Experiments for Plasma Biomarker Discovery

Cited by 201 publications

References 81 publications

Analysis of human serum phosphopeptidome by a focused database searching strategy

Analysis of human serum phosphopeptidome by a focused database searching strategy

Head-to-Head Comparison of Serum Fractionation Techniques

Structure and function of human plasma carboxypeptidase N, the anaphylatoxin inactivator

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