Identification of {alpha}1-Antitrypsin Variants in Plasma with the Use of Proteomic Technology

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

Articles

Identification of ${alpha}$ ₁-Antitrypsin Variants in Plasma with the Use of Proteomic Technology

Kevin Mills¹, Philippa B. Mills¹, Peter T. Clayton¹, Andrew W. Johnson¹, David B. Whitehouse² and Bryan G. Winchester¹^a

¹ Biochemistry Endocrinology and Metabolism Unit, Institute of Child Health at Great Ormond Street Hospital, University College London, 30 Guilford St., London WC1 N 1EH, United Kingdom.

² Medical Research Council Human Biochemical Genetics Unit, Galton Laboratory, University College London, London NW1 2HE, United Kingdom.

^aAuthor for correspondence. Fax 44-0207-404-6191; e-mail B.Winchester{at}ich.ucl.ac.uk.

Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Background: Proteomic technology permits the investigation ofgenetic metabolic diseases at the level of protein expression.Changes in the expression, polypeptide structure, and posttranslationalmodification of individual proteins can be detected in complexmixtures of proteins.

Methods: We used high-resolution two-dimensional polyacrylamidegel electrophoresis to separate isoforms of plasma proteinsand detect abnormalities of mass and/or charge. We confirmedthe identity of the separated proteins by in-gel digestion withproteases and N-glycanases and then analyzed the released peptidesand glycans by matrix-assisted laser-desorption ionization–time-of-flightmass spectrometry.

Results: Complete characterization of the polypeptide sequencesand glycosylation of ${alpha}$ ₁-antitrypsin isoforms was achieved inplasma from controls and from patients with three differentknown ${alpha}$ ₁-antitrypsin deficiencies and congenital disorder ofglycosylation type Ia.

Conclusions: This study shows that proteomic techniques area powerful and sensitive means of detecting changes in the aminoacid sequence and abnormal posttranslational modifications ofspecific proteins in a complex biologic matrix.

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The rapid expansion in proteomic research over the last 5 yearshas been brought about by the need to bridge the gap betweenthe sequence of a gene and the functional activity of its proteinproduct. The genome of a cell allows the prediction of the aminoacid sequence of a protein, but it does not indicate whetherthat protein is actually expressed or the extent of its expression(1). Some potential secondary and tertiary structural featuresand posttranslational motifs in a protein can be recognizedin a gene sequence. However, it is not possible to predict whetherthese features and motifs will be utilized in the mature functionalprotein unless the physiologic environment of its site of actionis known, i.e., the pattern of expression of proteins in itstissue of origin (2). Proteomics not only has the ability toprovide fundamental insights into the molecular basis of thephysiologic state of a cell, it also has the ability to revealhow cascades of protein expression change as a result of specificdisorders or drug treatment (3).

In the investigation of a genetic metabolic disorder causedby mutations in the gene encoding a protein (which may be anenzyme or transporter or structural protein), proteomic analysisshould be capable of the following: (a) detection of the alteredamino acid sequence in the mutated protein; (b) detection ofaltered posttranslational modification of the mutated proteinand other proteins; (c) measurement of the degree of expressionof the mutated protein and of other proteins involved in thepathogenesis of tissue damage; and (d) detection of polymorphismsin the mutated protein (which may modulate the mutation) andin other proteins (which may exacerbate or diminish the effectof the mutation by affecting the overall activity of the metabolicpathway involved). Given the number of proteins in tissue, theseare no small tasks.

This report examines two applications of proteomic technology:(a) the detection of mutant and polymorphic amino acid sequencesand (b) the detection of posttranslational modifications. Wehave chosen plasma ${alpha}$ ₁-antitrypsin as a target protein becauseplasma is readily available and is an important substrate forclinical investigation and because there are known diseasesthat result from changes in the amino acid sequence and theposttranslational modifications of ${alpha}$ ₁-antitrypsin [the ${alpha}$ ₁-antitrypsindeficiencies (4)]. A deficiency in ${alpha}$ ₁-antitrypsin can lead toemphysema in the third and fourth decades of life, and somedefects in ${alpha}$ ₁-antitrypsin [notably the protease inhibitor Z (PIZ) ¹ variant] can cause liver disease presenting in infancy or childhood(5)(6). The PIZ ${alpha}$ ₁-antitrypsin deficiency is the most commonmetabolic disease for which individuals currently undergo orthotopicliver transplantation (7). The primary function of ${alpha}$ ₁-antitrypsinis the inhibition of circulatory serine proteases or serpins,with the main target enzyme being neutrophil elastase, whichis found primarily in the lung (8). The pathophysiology of thelung disease has been explained by the deficiency of plasma ${alpha}$ ₁-antitrypsin, permitting an elastolytic attack on the lungby neutrophil elastase (9). The etiology of the liver diseasehas been more contentious (8)(9)(10). Most investigators believethat the amino acid substitution leads to the misfolding ofthe protein, leading to polymerization and a subsequent buildup of ${alpha}$ ₁-antitrypsin in the hepatocytes of the liver (9)(11)(12).However, little is known about the way in which this build upleads to inflammation and cirrhosis.

Mature ${alpha}$ ₁-antitrypsin has a molecular weight of M_r 52 000, consistsof a single polypeptide chain of 394 amino acids, and is $~$ 12%carbohydrate by weight (4). The ${alpha}$ ₁-antitrypsin molecule is synthesizedin the liver before secretion into the circulation where ithas a plasma concentration of $~$ 1.3 g/L (4) and a half-life of4–5 days (5). The ${alpha}$ ₁-antitrypsin molecule carries a highnegative charge because of sialic acid residues on the threecomplex glycans attached to asparagine residues 46, 83, and247 (13).

Isoelectric focusing of plasma ${alpha}$ ₁-antitrypsin leads to the detectionof eight bands, which are numbered M1 to M8 (anodal-low pH tocathodal-high pH) (14). The bands M4 and M6 are the most abundantof the isoforms, making up 40% and 34% of the total plasma ${alpha}$ ₁-antitrypsin,respectively, whereas M3 and M5 are present in only trace amounts(4). The multiple forms of ${alpha}$ ₁-antitrypsin are predominantly attributableto the presence of different numbers of sialic acid residuespresent on the glycans. Isoforms containing more triantennarycomplex glycans, and thus more sialic acid residues, have lowerpI values. Bands M4 and M6 have one triantennary plus two biantennaryglycans and three biantennary glycans, respectively (13). Thetwo minor cathodal isoforms, bands M7 and M8, have the samecarbohydrate structure as the major bands, M4 and M6, but M7and M8 lack the five N-terminal amino acids (Glu-Asp-Pro-Gln-Gly)(15). The loss of these five amino acids by posttranslationalcleavage causes an additional cathodal shift of the isoformsbecause of the loss of the negatively charged amino acids, glutamicacid (Glu 1) and aspartic acid (Asp 2) (15).

The combination of a well-characterized protein at a high concentrationin plasma and a well-characterized disease resulting from thedeficiency of that protein makes ${alpha}$ ₁-antitrypsin an ideal candidatefor this preliminary study in the application of proteomic techniquesto genetic metabolic disease. This report describes the proteomiccharacterization of ${alpha}$ ₁-antitrypsin from controls and the analysisof four ${alpha}$ ₁-antitrypsin variants resulting from changes in a singleamino acid in the sequence and/or posttranslational modifications.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

All chemical reagents used were of research grade and obtainedfrom Sigma-Aldrich, unless stated otherwise. Ultrapure electrophoretic-gradeacrylamide (30% by weight) was obtained from National DiagnosticsLtd. Anti- ${alpha}$ ₁-antitrypsin antibodies were coupled to Hi-Trap NHS-affinitychromatography columns (Amersham Pharmacia Biotech) accordingto the manufacturer’s instructions. Immobiline DryStripisoelectric focusing strips (18 cm; pH 4.5–5.5) were obtainedfrom Amersham Pharmacia Biotech. Piperazine diacrylamide cross-linkerwas obtained from Bio-Rad. All of the proteases used were ofsequence grade and were obtained from Promega Ltd. N-glycanaseand Glyco H graphite columns were obtained from Glyko.

molecular variants of ${alpha}$ ₁-antitrypsin
Plasma was obtained from four patients who had been diagnosedpreviously by biochemical and molecular genetic techniques withspecific alterations in the structure of ${alpha}$ ₁-antitrypsin (Fig.1 ).

View larger version (44K):
[in this window]
[in a new window]

Figure 1. Amino acid sequence of ${alpha}$ ₁-antitrypsin showing mutants analyzed in this study.

———, N-terminal amino acids (five); ${circ}$ , N-glycosylation sites 46, 83, and 247; , PIZ_Bristol (threonine⁸⁵ to methionine); ${square}$ , MIA²¹³ (valine²¹³ to alanine); ${diamond}$ , PIZZ (glutamate³⁴² to lysine).

Patient 1 was homozygous for a valine-to-alanine substitutionat amino acid 213 in ${alpha}$ ₁-antitrypsin, leading to a neutral aminoacid substitution (MIA²¹³).

Patient 2 was homozygous for a glutamate-to-lysine substitutionat amino acid 342 in ${alpha}$ ₁-antitrypsin, leading to a charged aminoacid substitution (PIZZ).

Patient 3 was homozygous for a deficiency in phosphomannomutase[congenital disorder of glycosylation type Ia (CDG-Ia)] (16),which causes underglycosylation of ${alpha}$ ₁-antitrypsin, leading toa change in molecular weight and charge.

Patient 4 was heterozygous for a C $->$ T transition at codon 85,which changes threonine 85 (ACG) to methionine (ATG) and abolishesthe N-glycosylation sequon (NLT) at amino acids 83–85,preventing glycosylation of asparagine 83 (PIZ_Bristol) (17).

gel electrophoresis
All two-dimensional polyacrylamide (2D-PAGE) analyses were performedaccording to Swiss-Prot protocols (18)(19)(20)(21)(22) withminor modifications.

one-dimension isoelectric focusing
We focused plasma samples for both analytical (2.5 µL)and preparative gels (10 µL for peptide mass fingerprintingand 30 µL for glycan analysis) on Immobiline DryStrips(18 cm; pH 4.5–5.5) using a LKB-Multiphor II focusingunit (Amersham Pharmacia Biotech). Isoelectric focusing wascarried out for a minimum of 75 kV h and a maximum of 100 kV·h.Focused strips were snap-frozen in liquid nitrogen and storedat -80 °C until later use.

two-dimension sodium dodecyl sulfate–page
Analytical gels consisted of 10% (by weight) acrylamide with1.6% cross-linker piperazine diacrylamide. We prepared preparativegels for in-gel proteolytic digestions using 10% (by weight)acrylamide with 0.1% or 1.3% bis-acrylamide for chymotrypsinand trypsin, respectively. We performed resolubilization ofthe focused proteins and carboamidomethylation of cysteine residuesaccording to Diettrich et al. (23). Sodium dodecyl sulfate–PAGEwas carried out in a Protean II Multicell electrophoresis unit(Bio-Rad).

detection of separated proteins
Analytical gels were silver-stained with an automatic gel stainer(Amersham Pharmacia Biotech) as described by Hochstrasser etal. (22), and the preparative gels were silver-stained accordingto Shevchenko et al. (24).

in-gel proteolytic digestion and extraction of peptides and glycans
In-gel tryptic digestions were performed as described by Shevchenkoet al. (24). In-gel chymotryptic digestions were performed ina similar manner but with the following minor modifications.The gel slices were incubated overnight with an excess of chymotrypsin(60 µL of 25 g/L), and the ammonium bicarbonate bufferwas replaced with 100 mmol/L Tris-HCl, pH 7.8. The releasedpeptides were extracted from the gel by shaking the gel sliceswith 300 µL of 50% acetonitrile containing 0.1% trifluoroaceticacid on a rotary mixer for 60 min. The acetonitrile was removedfrom the gel slice and taken down to dryness by centrifugalevaporation. Any residual peptides remaining in the gel slicewere extracted by shaking the gel slice with 300 µL of4 mol/L urea on a rotary mixer for 30 min. After the secondextraction, the urea solution was removed from the gel sliceand added to the dried peptides extracted with acetonitrile.This solution was vortex-mixed thoroughly for 60 s to resolubilizeall peptides before desalting on a C-18 stationary-phase microcolumnas described by Mills et al. (25). The desalted peptide solutionwas dried by centrifugal evaporation and reconstituted in 10µL of 1 mL/L trifluoroacetic acid for mass spectrometry.

Preparative gels for glycan analysis were stained with Coomassieblue, and glycans were released by in-gel digestion with PNGaseF according to Kuster et al. (26). The released glycans weredesalted with graphite Glyco H columns (Glyko) before analysisby mass spectrometry.

identification of proteins separated by 2d-page
Proteins separated by 2D-PAGE were identified by mass-mappingstudies (see below). The pI and molecular weight coordinatesfor our 2D-PAGE system were then determined by comparison ofthe identified proteins with the Swiss-Prot online plasma 2D-PAGEdatabase (Geneva, Switzerland; http://www.expasy.ch/cgi bin/map2/def?PLASMA_HUMAN).

mass spectrometry
Mass spectrometry was carried out on a matrix-assisted laserdesorption ionization–time-of-flight mass spectrometry(MALDI-TOF-MS) instrument fitted with a reflectron and a 337-nmultraviolet laser (TOF Spec E; MicroMass). Peptide analyseswere performed in positive-ion mode with the following voltages:source, 20 kV; extraction, 19.95 kV; focus, 16.5 kV; and reflectron,25 kV. Spectra were acquired by calculating the mean value offive scans with the highest signal. Data were acquired in reflectronmode, operating over a mass range of m/z 6000 with matrix suppressionset at 650 Da. Peptides were analyzed with an ${alpha}$ -cyano-4-hydroxycinnamicacid–fucose comatrix as described by Mills et al. (25).

Glycan analyses were performed in negative-ion mode with voltagesof 20 kV for the source, 19.95 kV for the extraction, 16.5 kVfor the focus, and a pulse voltage of 900 V. Spectra were acquiredby calculating the mean value of five scans with the highestsignal. Data were acquired in linear mode, operating over amass range of m/z 4000 with matrix suppression set at 800 Da.Glycans were analyzed with trihydroxyacetophenone–20 mmol/Lammonium citrate comatrix according to Papac et al. (27).

Data analysis was carried out with MassLynx data analysis software(Protein Prospector database software, the University of SanFrancisco; http://falcon.ludwig.ucl.ac.uk/mshome3.2.htm) andPAWS proteomic analysis software.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

2D-PAGE analysis of control plasma indicated the presence ofsix putative isoforms of ${alpha}$ ₁-antitrypsin on the basis of theirpI value and size (Fig. 2A ). Tryptic peptide mass mapping confirmedthat all of these components were ${alpha}$ ₁-antitrypsin and identifiedseveral other proteins. Variation in the electrophoretogramsfor healthy subjects was extensively studied. No changes inthe expression or the ratio of pI/M_r were observed in any ofthe 2D-PAGE analyses of the many control plasmas analyzed. Theexpression of the ${alpha}$ ₁-antitrypsin was remarkably consistent amongthe control individuals, and the electrophoretogram includedis representative of a typical 2D-PAGE pattern for ${alpha}$ ₁-antitrypsinin control plasma samples. Several control samples were analyzedat the same time as every ${alpha}$ ₁-antitrypsin variant to avoid batch-to-batchdifferences during electrophoresis and staining. The preciseidentity of each isoform was deduced from glycan analysis andthe intensity and peptide mass spectra of the isoform. Peptidemass mapping of the two most abundant isoforms, the putativeM4 and M6 isoforms, with trypsin and chymotrypsin, respectively,showed the presence of peptides of masses m/z 2819.2 and m/z3704.7, respectively (Fig. 3, A and B ). These masses correspondto peptides containing the amino acids 1–25 and 1–33,respectively, in the sequence of ${alpha}$ ₁-antitrypsin and indicatethat these isoforms do contain the first five amino acids, aspredicted by Jeppsson et al. (15). Both of these peptides containmissed cleavage sites at lysine 10 and phenylalanine 23, respectively.No ions corresponding to peptides containing the five N-terminalamino acids were observed in the analysis of the predicted M7(Fig. 3C ) and M8 isoforms (Fig. 3D ), supporting their identification.However, a tryptic peptide mass (m/z 1779.8) corresponding toresidues 11–26 was detected. We postulate that trypticcleavage after lysine 10 occurs more readily in the truncatedprotein than in the intact protein, preventing the appearanceof a peptide corresponding to residues 6–25 (m/z 2293.0).The use of the two proteases independently increased the coverageof the amino acid sequence to 86% from 65.2% and 52.3% for trypsinand chymotrypsin, respectively.

View larger version (89K):
[in this window]
[in a new window]

Figure 2. Analytical 2D-PAGE of control and MIA²¹³ plasma samples and a sample from a heterozygote for PIMZ_Bristol.

Enlarged 2D-PAGE sections of plasma ${alpha}$ ₁-antitrypsin (A), MIA²¹³ plasma ${alpha}$ ₁-antitrypsin (B), and plasma ${alpha}$ ₁-antitrypsin from a heterozygote for PIMZ_Bristol (C) within a narrow pH range of 4.5–5.5 for focusing in the first dimension. Ordinate values are M_r of known proteins. (C), spots 1–4 show additional ${alpha}$ ₁-antitrypsin isoforms.

View larger version (23K):
[in this window]
[in a new window]

Figure 3. MALDI-TOF-MS of tryptic and chymotryptic digests of ${alpha}$ ₁-antitrypsin isoforms in control plasma.

(A), tryptic digest of the M4 isoform showing a peptide of m/z 2819.2, corresponding to amino acids 1–25. (B), chymotryptic digest of the M6 isoform showing a peptide of m/z 3704.7, corresponding to amino acids 1–33. (C), tryptic digest of the M7 isoform showing no extra peptides corresponding to amino acids 1–25 in the sequence. (D), chymotryptic digest of the M8 isoform showing no extra peptides corresponding to amino acids 1–33 in the sequence.

Further evidence for the identity of the major isoforms M4 andM6 was obtained by analysis of glycans released by in-gel digestionwith PNGase F. Fig. 4A shows the glycan analysis of the M4isoform. Two major glycans were detected, disialo-biantennary(m/z 2223.4) and trisialo-triantennary (m/z 2880.1), in a ratioof $~$ 2:1. The next most abundant peak, m/z 1932.2, is probablyattributable to in-source loss of sialic acid from the majorbiantennary glycan. Masses corresponding to fucosylated bi-(m/z 2369.6) and triantennary (m/z 3026.3) structures were alsoobserved and constituted 5% and 7% of the total glycan signal,respectively. The glycan analysis of the predicted M6 isoformshowed the presence of only one major species, the disialo-biantennarycomplex glycan structure (Fig. 4B ). As with the analysis ofthe M4 spot, a mass corresponding to a fucosylated biantennarystructure was also observed, which constituted $~$ 8% of the totalglycan signal.

View larger version (23K):
[in this window]
[in a new window]

Figure 4. MALDI-TOF-MS of glycans released from ${alpha}$ ₁-antitrypsin isoforms.

Mass spectra of the glycans obtained from the in-gel N-glycanase digestion of the M4 (A) and M6 (B) isoforms of ${alpha}$ ₁-antitrypsin.

These results are in accord with previously published data forthe microheterogeneity of glycosylation of the major isoformsof ${alpha}$ ₁-antitrypsin in human plasma (13)(14)(15). The M4 isoformof ${alpha}$ ₁-antitrypsin has been reported previously to contain twobiantennary and one triantennary complex glycan, which is inagreement with our observation of bi- to triantennary glycansin a ratio of 2:1 (4). Similarly, our detection of only biantennaryglycans on M6 agrees with the data published by Jeppsson etal. (12). Naitoh et al. (28) reported that the M4 and M6 ${alpha}$ ₁-antitrypsinisoforms contain small amounts of fucosylated glycans, whichagain is in agreement with our observations.

The glycosylation analyses for the putative M7 and M8 isoformswere the same as those for the M4 and M6 isoforms, respectively,confirming that their different pI values were attributableto the loss of the five N-terminal amino acids and not to adifference in glycosylation.

Unfortunately, the mass spectral signals for the analyses ofthe glycans on the M1 and M2 isoforms of ${alpha}$ ₁-antitrypsin wereextremely weak, and it was not possible to identify the microheterogeneityof the glycosylation of these isoforms unequivocally. Peptideanalyses from these spots indicated that the first five aminoacids in the ${alpha}$ ₁-antitrypsin sequence were present in both ofthese isoforms. The presence of the first five amino acids indicatesthat the different pI values of these isoforms must be attributableto glycan heterogeneity and not to posttranslational proteolysis.We therefore postulate that the isoforms M1 and M2 contain threetriantennary glycans and two tri- plus one biantennary glycan,respectively, for the isoforms to migrate to the pI values observedwith 2D-PAGE.

The use of high-resolution isoelectric focusing over the pHrange 4.5–5.5 permitted complete separation of the isoformsof ${alpha}$ ₁-antitrypsin, which was not possible with the use of widerpH ranges of ampholines. The ability to "focus" on particularpH ranges allows greater resolution of individual proteins and,more significantly, increases the probability of resolving theprotein of interest from other proteins of similar pI and massfor analysis by mass spectrometry. The combination of glycananalysis to determine the microheterogeneity of glycosylationand peptide mass fingerprinting permitted the accurate identificationof the abundant isoforms, M4, M6, M7, and M8, and a reasonableprediction of the structure of the M1 and M2 isoforms of ${alpha}$ ₁-antitrypsinseparated by 2D-PAGE (see Fig. 2A ).

analysis of molecular variants of ${alpha}$ ₁-antitrypsin
Neutral amino acid substitution (V213A).
No marked changes in the protein intensity, pI, or molecularweight of the ${alpha}$ ₁-antitrypsin isoforms were observed when the2D-PAGE analyses of control plasma samples were compared withpatient (V213A) plasma samples (Fig. 2, A and B , respectively).This is consistent with a neutral amino acid substitution, whichwould not be expected to alter the physical characteristicsof ${alpha}$ ₁-antitrypsin.

The MALDI-TOF-MS analyses of the tryptic digests of the controland patient ${alpha}$ ₁-antitrypsin isoforms were similar, except forthe fragment corresponding to the tryptic peptide containingamino acids 192–217. Masses of m/z 3148.5 and m/z 3120.5were observed from the each ${alpha}$ ₁-antitrypsin equivalent isoformfrom the control and V231A variant isoforms, respectively (Fig.5, A and B , respectively). These masses differ by 28 m/z andare consistent with a peptide containing a valine-to-alaninesubstitution at residue 213 in the variant. The mass of m/z3148.5 derived from the control ${alpha}$ ₁-antitrypsin was not observedin the ${alpha}$ ₁-antitrypsin from the V213A patient and vice versa.

View larger version (28K):
[in this window]
[in a new window]

Figure 5. MALDI-TOF-MS of the tryptic in-gel digestion of control, MIA²¹³, and PIZZ (GLU³⁴²) ${alpha}$ ₁-antitrypsin.

(A), tryptic in-gel digest of the control M4 isoform showing a peptide of mass m/z 3148.5, corresponding to amino acids 199–217 containing valine at position 213. (B), tryptic in-gel digest of the MIA²¹³ M4 isoform showing a peptide of mass m/z 3120.5, corresponding to amino acids 199–217 containing alanine at position 213. (C), enlarged 2D-PAGE section of control plasma ${alpha}$ ₁-antitrypsin within a narrow pH range of 4.5–5.5. (D), enlarged 2D-PAGE section of PIZZ (GLU³⁴²) plasma ${alpha}$ ₁-antitrypsin within a narrow range pH 4.5–5.5.

Charged amino acid substitution (E342K): PIZ variant.
The 2D-PAGE analysis of PIZZ patient plasma showed changes inthe intensity and pI of all the ${alpha}$ ₁-antitrypsin isoforms relativeto the control plasma sample (Fig. 6, A and B ). The intensitiesof the main M4 and M6 isoforms in the PIZZ plasma were $~$ 20% ofthe intensities of the equivalent spots in the control plasma.The concentration of ${alpha}$ ₁-antitrypsin in PIZZ plasma has been reportedby Sveger et al. (29) to be 17% ± 3% of that in nondiseasedplasma. The six ${alpha}$ ₁-antitrypsin isoforms in the PIZZ plasma showeda cathodal shift relative to their counterparts in control plasma.The mean cathodal shift in pI between each of the PIZZ isoformsand its equivalent control isoform was 0.1 pH units. This isapproximately double the pI difference observed between adjacentisoforms in the same plasma sample (0.05 pH units), which differby one sialic acid residue or one negative charge. Thus theincrease in pI of each PIZZ isoform relative to its controlcounterpart can be explained by the substitution of a positivelycharged lysine residue for a negatively charged glutamate residuewith a net decrease in negative charge of 2, which is equivalentto an increase in pI of $~$ 0.1 pH units.

View larger version (76K):
[in this window]
[in a new window]

Figure 6. Analytical 2D-PAGE of control and PIZ plasma.

Enlarged 2D-PAGE section of control plasma ${alpha}$ ₁-antitrypsin (A) and PIZZ (GLU³⁴²) plasma ${alpha}$ ₁-antitrypsin (B) within a narrow pH range of 4.5–5.5.

As the concentration of ${alpha}$ ₁-antitrypsin in PIZZ plasma is quitelow, it was initially purified by immunoaffinity chromatographyfollowed by one-dimensional PAGE to optimize the digestion conditionsfor analysis by mass spectrometry. A small amount of contaminatingalbumin (confirmed by mass mapping) was detected in the one-dimensionalPAGE, but it was clearly resolved from the ${alpha}$ ₁-antitrypsin. Theseparated ${alpha}$ ₁-antitrypsin was digested in-gel with trypsin andthe resulting peptide mixture analyzed by MALDI-TOF-MS. Onlypeptides containing a lysine residue at position 342, as opposedto a glutamate, were detected in the analysis.

Having defined the digestion and mass spectrometry conditionsfor detection of the amino acid change, we applied these conditionsto the ${alpha}$ ₁-antitrypsin isoforms separated by 2D-PAGE. The spectraobserved from the in-gel digestion of isoform M4 in the controland PIZZ plasma samples over the mass range m/z 2020–2640are shown in Fig. 5, C and D , respectively. Three extra masses,m/z 2387.2, m/z 2403.2, and m/z 2419.2, were observed in thePIZZ ${alpha}$ ₁-antitrypsin analysis, which were not observed in thecontrol analysis. These masses correspond to a peptide coveringamino acids 343–365 in the sequence of ${alpha}$ ₁-antitrypsin aftercleavage between the two lysine residues at positions 342 and343. The observation of three masses for a single peptide isexplained by the presence of the same peptide in the three forms,i.e., native (m/z 2387.2) and with one (m/z 2403.2) or two (m/z2419.2) oxidized methionine residues. This confirmed that thePIZZ patient was homozygous for the E342K mutation. No peptidecovering amino acids 343–365 in the sequence was detectedin the analysis of the control plasma. An ion correspondingto residues Ala-336–Lys- 342 (m/z 887.6) could not bedetected because it would fall into the matrix noise signalobserved on the mass spectrometer. A possible explanation forthe detection of a peptide covering the mutation region in thePIZZ sample, but not in the control, could be the nature ofthe amino acid substitution. The substitution of a lysine fora glutamate residue adjacent to another lysine residue at aminoacid 343 creates a highly positively charged dilysine motifin the variant. This would be expected to enhance tryptic cleavagebetween the two lysines. In contrast, the negatively chargedglutamic acid at position 342 in the normal sequence would beexpected to inhibit cleavage after lysine 343. In fact, thisarea of the sequence is intransigent to in-gel tryptic digestioneven after prior deglycosylation (25). The three extra massesof native m/z 2387.2, m/z 2403.2, and m/z 2419.2 were foundin all the ${alpha}$ ₁-antitrypsin isoforms from the PIZ variant but notin the control.

underglycosylation
CDG type I results from a deficiency of phosphomannomutase,which leads to a decreased capacity for asparagine-linked glycosylationof proteins. An important diagnostic manifestation of CDG-Iais the appearance of more cathodal glycoforms of plasma/serumglycoproteins on electrophoresis attributable to their underglycosylationand consequent loss of sialic acid residues. Seven extra ${alpha}$ ₁-antitrypsinisoforms (spots 1a–7a) were observed in the 2D-PAGE analysisof plasma from a patient with CDG-Ia (Fig. 7A ). These wereanalyzed by peptide mass fingerprinting to establish the molecularbasis of their different pI values and masses. Spots 1a–5aall had M_r $~$ 2000 less than the corresponding M series of ${alpha}$ ₁-antitrypsinisoforms in control plasma, which were also present in the CDG-Iaplasma sample (Fig. 7A ). This decrease in mass is consistentwith the loss of one complex N-linked glycan. Spots 6a and 7ahad a M_r $~$ 4000 less than the control M series, consistent withthe loss of two complex glycans. These mass differences suggestthat isoforms 1a-7a are underglycosylated compared with thecontrol M isoforms.

View larger version (56K):
[in this window]
[in a new window]

Figure 7. 2D-PAGE and mass spectra of plasma ${alpha}$ ₁-antitrypsin from CDG, control, and PIMZ_Bristol plasma.

(A), 2D-PAGE of CDG plasma ${alpha}$ ₁-antitrypsin and mass spectra of the tryptic in-gel digestion of spot 3a, showing a peptide of mass m/z 3691.8, corresponding to amino acids 70–101 with an asparagine at position 83. (B), 2D-PAGE of control plasma ${alpha}$ ₁-antitrypsin and mass spectra of the tryptic in-gel digestion of the M6 isoform after prior enzymatic removal of the glycans. A new peptide of mass m/z 3692.8 corresponding to amino acids 70–101 with an aspartic acid at position 83 is observed. (C), 2D-PAGE of control plasma ${alpha}$ ₁-antitrypsin and mass spectra of the tryptic in-gel digestion of the M6 isoform. (D), 2D-PAGE of PIMZ_Bristol plasma ${alpha}$ ₁-antitrypsin and mass spectra of the tryptic in-gel digestion of spot 3, showing a peptide of m/z 3737.8, corresponding to amino acids 70–101 with an asparagine at position 83 and a methionine at position 85.

The state of glycosylation of spots 1a–7a was investigatedby mass mapping studies. It has been shown previously (25) thatglycopeptides containing complex glycans do not produce detectableions under the conditions used here for mass spectrometry, whereasthe same peptides in which the asparagine is not glycosylatedor in which the asparagine has been converted to aspartic acidby enzymatic deglycosylation can be detected (Fig. 7B ). Theseobservations provide a means for assessing the occupancy ofa glycosylation site.

An extra mass at m/z 3691.8, which was not detected in the controlM series of ${alpha}$ ₁-antitrypsin, was detected in all of the trypticpeptide maps of spots 1a–5a (Fig. 7A ). The mass of m/z3691.8 corresponds to the peptide containing amino acids 70–101with an asparagine residue at amino acid 83, which indicatesthat this glycosylation site is not occupied (Fig. 7A ). Massescorresponding to peptides containing asparagine at the two otherglycosylation sites, asparagines 46 and 247, were not detected,implying that these glycosylation sites were occupied. Thusthe decrease in mass and increase in pI of spots 1a–5aare probably attributable to nonglycosylation of asparagine83. This unglycosylated peptide (70–101) was also presentin the tryptic peptide map of spots 6a and 7a, together withmass of m/z 1755.9, which is also absent from the control isoforms.This mass corresponds to a peptide covering the amino acids244–259 with asparagine at position 247. These data indicatethat the isoforms 6a and 7a are glycosylated only at asparagine46 and that this accounts for their positions on 2D-PAGE.

altered amino acid sequence and posttranslational modification
The 2D-PAGE analysis of the plasma from the PIMZ_Bristol heterozygote(Fig. 2C ) revealed the presence of four additional putative ${alpha}$ ₁-antitrypsin isoforms that were not present in the controlplasma (Fig. 2A ). All four of these additional spots were identifiedas ${alpha}$ ₁-antitrypsin by mass mapping studies. Spots 1, 2, 3, and4 had pI values of 5.07, 5.10, 5.16, and 5.27, respectively,and M_r $~$ 2000 less than the control M series of ${alpha}$ ₁-antitrypsinisoforms. These changes in pI and mass are consistent with theloss of a complex biantennary glycan, as was seen in some ofthe ${alpha}$ ₁-antitrypsin isoforms in CDG-Ia. The substitution of amethionine for threonine at position 85 in PIMZ_Bristol ${alpha}$ ₁-antitrypsinleads to the loss of a sequon for N-linked glycosylation, i.e.,NLT⁸⁵E $->$ NLM⁸⁵E. The loss of this sequon would be expected to leadto isoforms of ${alpha}$ ₁-antitrypsin that are not glycosylated at asparagine83 and have only two of the three glycosylation sites occupied.The observed changes in pI and molecular weight suggest thatthe four novel isoforms contain the PIZ_Bristol mutation. Thepresence of two sets of isoforms in the 2D-PAGE shows that boththe wild-type (M) and variant alleles of ${alpha}$ ₁-antitrypsin are expressedin the plasma of PIMZ_Bristol heterozygotes and can be detectedby this protocol.

To demonstrate that the novel isoforms 1–4 were attributableto the PIMZ_Bristol allele, we subjected them to in-gel digestionwith trypsin followed by mass spectrometry of the resultingpeptide mixture. An additional mass of m/z 3737.8 was detectedin each of the isoforms (Fig. 7D ), which was not present inthe M series of ${alpha}$ ₁-antitrypsin in both the PIMZ_Bristol heterozygoteand the control (Fig. 7C ). A peptide of m/z 3737.8 can be accountedfor by a peptide containing amino acids 70–101 with methionineat position 85 and asparagine at position 83, i.e., it is derivedfrom the PIMZ_Bristol allele with a nonglycosylated asparagine83. The lack of glycosylation at asparagine 83 permits in-geltryptic digestion of this region, as was seen in the underglycosylatedisoforms from CDG-Ia. A glycopeptide covering sequon 83 wasnot observed in any of the M series of ${alpha}$ ₁-antitrypsin isoformsfrom control or mutant samples. This is attributable to thedifficulty of analyzing complex sialic acid-containing glycopeptideswith MALDI-TOF-MS. We obtained further evidence that a peptidecontaining amino acids 70–101 can be produced by trypticdigestion and detected by MALDI-TOF-MS if it is not glycosylatedby N-glycanase to remove glycans before mass mapping studies.A peptide of mass m/z 3692.8 was detected in the mass spectrumafter in-gel tryptic digestion of the main M4 isoform afterprior enzymatic removal of the glycans with N-glycanase F (Fig.7B ). This mass corresponds to a peptide covering amino acids70–101 in the sequence, but with an aspartic acid residueat position 83. The mass of this peptide (m/z 3692.8) is onemass unit greater than the mass of the unglycosylated peptide(m/z 3691.8) that contains amino acids 70–101 found in ${alpha}$ ₁-antitrypsin from CDG-Ia because of the conversion of an asparagine83 to aspartic acid during the release of the glycan by theN-glycanase.

Further characterization of the novel isoforms 1, 2, 3, and4 was obtained by analysis of their N-terminal peptides andglycans. The major mutant isoforms, spots 2 and 3 (Fig. 7D ),both had the same glycan profile as the control M4 and M6 isoforms(Fig. 2A ). The peptide analysis of spots 2 and 3 also containedmasses corresponding to amino acids 1–20 in the aminoacid sequence. Therefore, spots 2 and 3 are the equivalentsof the major control M4 and M6 isoforms but lack glycosylationat asparagine 83. The combined glycan and peptide analysis ofspot 4 showed that it was the unglycosylated equivalent of thecontrol M8 isoform of ${alpha}$ ₁-antitrypsin. It was not possible tocarry out glycan analysis of spot 1, but its pI and mass suggestthat it is the equivalent of the normal M2 isoform. Thus themutant spots 1, 2, 3, and 4 observed in the PIZ_Bristol plasmaare the underglycosylated (at asparagine 83) equivalents ofthe M2, M4, M6, and M8 isoforms of ${alpha}$ ₁-antitrypsin. The reasonfor the absence of an equivalent to the M7 ${alpha}$ ₁-antitrypsin isoformin the PIMZ_Bristol plasma is not clear. It could be that itis not secreted from the liver as in the PIZZ phenotype wheredecreased amounts of mutant ${alpha}$ ₁-antitrypsin are observed in theplasma. However, only the mutant M7 isoform was absent fromthe plasma samples of the PIZ_Bristol heterozygotes, whereasall isoforms were observed, albeit in decreased amounts, inthe plasma of PIZZ patients.

Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

We believe this work is a good example of the usefulness ofproteomics as a tool in the detection and further understandingof genetic metabolic diseases. Proteomics is a natural developmentof the pioneering work on the 2D-PAGE separation of multipleforms of ${alpha}$ ₁-antitrypsin (30)(31).

However, it is important to recognize the limitations of proteomicmethodology. As reported previously (25), the use of two ormore proteases may be required to obtain peptides that coverthe complete amino acid sequence of a protein. Analysis of ${alpha}$ ₁-antitrypsinby in-gel tryptic digestion allows only $~$ 60% of the amino acidsequence to be covered. However, when we used chymotrypsin aswell, it was possible for us to cover 86% of the sequence. Allthe mutations analyzed in this study were chosen deliberatelyto be in peptides produced by in-gel tryptic digestion.

This study shows that it is possible to detect known alterationsin the amino acid sequence of a protein with the use of MALDI-TOF-MSto detect a peptide that is not present in the digestion ofthe normal protein. Reliable detection of unknown amino acidsubstitutions will require sequencing of all the peptides generatedby proteolytic digestion of the protein. Although MALDI-TOF-MShas the capability of sequencing peptides by postsource decayanalysis, sequencing can be carried out more efficiently andsensitively with a quadrupole time-of-flight mass spectrometer,such as the Q-TOF (MicroMass) or ion-trap mass spectrometer.

The data generated in this study were essentially qualitative.To derive the maximum information from proteomic analysis itwill be important to be able to quantify the degree of expressionof all the important proteins. Methods need to be developedto ensure that all peptides are sequenced and measured quantitativelyfor the reliable detection of mutations and measurement of thedegree of expression of proteins in a metabolic pathway. Priorimmunoprecipitation of less abundant proteins could be usedto increase the sensitivity of this strategy.

Acknowledgments

We would like to thank Drs. Kevin Rogers and Richard Tyldesleyof MicroMass UK for help with the mass spectrometry and Dr.Ole Diettrich for advice and refinements to the 2D-PAGE protocol.We would also like to thank Dr. Ted Tarelli for help and advicein the analysis of glycans by MALDI-TOF-MS. The financial supportof the Wellcome Trust, the Sir Jules Thorn Charitable Trustand the European Union (Euroglycan) are gratefully acknowledged.Research at the Institute of Child Health and Great Ormond StreetHospital for Sick Children NHS Trust benefits from R & Dfunding received from the NHS Executive.

Footnotes

¹ Nonstandard abbreviations: PI, protease inhibitor; CDG-Ia, congenitaldisorder of glycosylation type Ia; 2D-PAGE, two-dimensionalpolyacrylamide gel electrophoresis; and MALDI-TOF-MS, matrix-assistedlaser desorption–ionization time-of-flight mass spectrometry.

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Humphery-Smith I, Blackstock W. Proteome analysis: genomics via the output rather than the input code. J Protein Chem 1997;16:537-544.[Web of Science][Medline] [Order article via Infotrieve]
Varki A. Biological roles of oligosaccharides: all of the theories are correct?. Glycobiology 1993;3:97-130.[Abstract/Free Full Text]
Parekh R. Proteomics and molecular medicine. Nat Biotechnol 1999;17:19-20.[Web of Science][Medline] [Order article via Infotrieve]
Cox DW. ${alpha}$ ₁-Antitrypsin deficiency. 7th ed. Scriver CR Beaudet AC Sly WS Valle D eds. The metabolic and molecular bases of inherited diseases 1995;Vol. III:4125-4158 McGraw-Hill New York. .
Brantly M, Nukiwa T, Crystal RG. Molecular basis of ${alpha}$ ₁-antitrypsin. Am J Med 1988;84:13-31.[Web of Science][Medline] [Order article via Infotrieve]
Eriksson S. ${alpha}$ ₁-Antitrypsin deficiencies. Acta Med Scand 1964;175:197-205.[Web of Science][Medline] [Order article via Infotrieve]
Sherlock S, Dooley J. Hepatic transplantation. Diseases of the liver and biliary system 9th ed. 1992:613-620 Blackwell Scientific Publications Oxford, United Kingdom. .
Travis J, Salvesen GS. Human plasma proteinase inhibitors. Ann Rev Biochem 1983;52:655-709.[Web of Science][Medline] [Order article via Infotrieve]
Kim D, Yu MH. Folding pathway of human ${alpha}$ ₁-antitrypsin. Biochem Biophys Res Commun 1996;226:378-384.[Web of Science][Medline] [Order article via Infotrieve]
Bathurst IC, Travis J, George PM, Carrell RW. Structural and functional characterisation of the abnormal Z ${alpha}$ ₁-antitrypsin isolated from human liver. FEBS Lett 1984;177:179-183.[Web of Science][Medline] [Order article via Infotrieve]
Foreman RC. Disruption of the Lys290-Glu342 salt bridge in human ${alpha}$ ₁-antitrypsin isolated from human liver does not prevent its synthesis or secretion. FEBS Lett 1987;216:79-82.[Web of Science][Medline] [Order article via Infotrieve]
Bottomley SP, Chang WS. The effect of the reactive centre loop length upon serpin polymerisation. Biochem Biophys Res Commun 1997;241:264-269.[Web of Science][Medline] [Order article via Infotrieve]
Vaughan L, Lorier M, Carrell RW. ${alpha}$ ₁-Antitrypsin microheterogeneity: isolation and the physiological significance of isoforms. Biochim Biophys Acta 1982;701:339-345.[Medline] [Order article via Infotrieve]
Fagerhol MK, Laurell CB. The polymorphism of ‘prealbumins’, ${alpha}$ ₁-antitrypsin in human sera. Clin Chim Acta 1967;16:199-203.[Web of Science][Medline] [Order article via Infotrieve]
Jeppsson JO, Lilja H, Johansson M. Isolation and characterization of 2 minor fractions of ${alpha}$ ₁-antitrypsin by high performance liquid chromatography chromatofocusing. J Chromatogr 1985;327:173-177.[Web of Science][Medline] [Order article via Infotrieve]
Keir G, Winchester BG, Clayton PT. Carbohydrate-deficient glycoprotein syndromes: inborn errors of protein glycosylation. Ann Clin Biochem 1999;36:20-36.
Lovegrove J, Jeremiah D, Gillet GT, Temple IK, Povey S, Whitehouse DB. A new ${alpha}$ ₁-antitrypsin mutation, THR-MET85 (PIZ_Bristol), associated with novel electrophoretic properties. Ann Hum Genet 1997;61:385-391.[Web of Science][Medline] [Order article via Infotrieve]
Hughes GJ, Frutiger S, Paquet N, Ravier F, Pasquali C, Sanchez JC, et al. Plasma protein map–an update by microsequencing. Electrophoresis 1992;13:707-714.[Web of Science][Medline] [Order article via Infotrieve]
Bjellqvist B, Pasquali C, Ravier F, Sanchez J-C, Hochstrasser DF. A nonlinear wide range immobilized pH gradient for 2D-PAGE and its definition in a relevant pH scale. Electrophoresis 1993;14:1357-1365.[Web of Science][Medline] [Order article via Infotrieve]
Hochstrasser DF, Patchornik A, Merril CR. Development of polyacrylamide gels that improve the separation of proteins and their detection by silver staining. Anal Biochem 1988;173:412-423.[Web of Science][Medline] [Order article via Infotrieve]
Hochstrasser DF, Merril CR. Catalysts’ for polyacrylamide gel polymerization and detection of proteins by silver staining. Appl Theor Electrophor 1988;1:35-40.[Medline] [Order article via Infotrieve]
Hochstrasser DF, Harrington MG, Hochstrasser AC, Miller MJ, Merril CR. Methods for increasing the resolution of two-dimensional protein electrophoresis. Anal Biochem 1988;173:424-435.[Web of Science][Medline] [Order article via Infotrieve]
Diettrich O, Mills K, Johnson AW, Hasilik A, Winchester BG. Application of magnetic chromatography to the isolation of lysosomes from fibroblasts of patients with lysosomal storage disorders. FEBS Lett 1998;441:369-372.[Web of Science][Medline] [Order article via Infotrieve]
Shevchenko A, Wilm M, Vorm O, Mann M. Mass spectrometric sequencing of proteins from silver stained polyacrylamide gels. Anal Chem 1996;68:850-858.[Medline] [Order article via Infotrieve]
Mills K, Johnson AW, Clayton PT, Diettrich OGP, Winchester BG. A strategy for the identification of site specific glycosylation in glycoproteins using MALDI TOF MS. Tetrahedron Asymmetry 2000;11:75-93.
Kuster B, Hunter AP, Wheeler SF, Dwek RA, Harvey DJ. Structural determination of N-linked carbohydrates by matrix-assisted laser desorption/ionization-mass spectrometry following enzymatic release within sodium dodecyl sulphate-polyacrylamide electrophoresis gels: application to species-specific glycosylation of ${alpha}$ ₁-acid glycoprotein. Electrophoresis 1998;19:1950-1959.[Web of Science][Medline] [Order article via Infotrieve]
Papac DI, Wong A, Jones AJ. Analysis of acidic oligosaccharides and glycopeptides by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. Anal Chem 1996;15:3215-3223.
Naitoh A, Aoyagi Y, Asakura H. Highly enhanced fucosylation of serum glycoproteins in patients with hepatocellular carcinoma. J Gastroenterol Hepatol 1999;14:436-445.[Web of Science][Medline] [Order article via Infotrieve]
Sveger T. Plasma protease inhibitors in ${alpha}$ ₁-antitrypsin deficient children. Pediatr Res 1985;19:834-835.[Web of Science][Medline] [Order article via Infotrieve]
O’Farrell PH. High resolution two-dimensional electrophoresis of proteins. J Biol Chem 1974;250:4007-4021.[Abstract/Free Full Text]
Anderson L, Anderson NG. High resolution two-dimensional electrophoresis of human plasma proteins. Proc Natl Acad Sci U S A 1977;74:5421-5425.[Abstract/Free Full Text]

The following articles in journals at HighWire Press have cited this article:

B. B. Cheung, J. Bell, A. Raif, A. Bohlken, J. Yan, B. Roediger, A. Poljak, S. Smith, M. Lee, W. D. Thomas, et al.
The Estrogen-responsive B Box Protein Is a Novel Regulator of the Retinoid Signal
J. Biol. Chem., June 30, 2006; 281(26): 18246 - 18256.
[Abstract] [Full Text] [PDF]

Y. Wang, S.-l. Wu, and W. S. Hancock
Approaches to the study of N-linked glycoproteins in human plasma using lectin affinity chromatography and nano-HPLC coupled to electrospray linear ion trap--Fourier transform mass spectrometry
Glycobiology, June 1, 2006; 16(6): 514 - 523.
[Abstract] [Full Text] [PDF]

B. Thomsen, P. Horn, F. Panitz, E. Bendixen, A. H. Petersen, L.-E. Holm, V. H. Nielsen, J. S. Agerholm, J. Arnbjerg, and C. Bendixen
A missense mutation in the bovine SLC35A3 gene, encoding a UDP-N-acetylglucosamine transporter, causes complex vertebral malformation
Genome Res., January 1, 2006; 16(1): 97 - 105.
[Abstract] [Full Text] [PDF]

L. Valmu, A. Paju, M. Lempinen, E. Kemppainen, and U.-H. Stenman
Application of Proteomic Technology in Identifying Pancreatic Secretory Trypsin Inhibitor Variants in Urine of Patients with Pancreatitis
Clin. Chem., January 1, 2006; 52(1): 73 - 81.
[Abstract] [Full Text] [PDF]

E. Ballot, A. Bruneel, V. Labas, and C. Johanet
Identification of Rat Targets of Anti-Soluble Liver Antigen Autoantibodies by Serologic Proteome Analysis
Clin. Chem., April 1, 2003; 49(4): 634 - 643.
[Abstract] [Full Text] [PDF]

K. Mills, P. B. Mills, P. T. Clayton, N. Mian, A. W. Johnson, and B. G. Winchester
The underglycosylation of plasma {alpha}1-antitrypsin in congenital disorders of glycosylation type I is not random
Glycobiology, February 1, 2003; 13(2): 73 - 85.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (21)

Citing Articles via Google Scholar

Google Scholar

Articles by Mills, K.

Articles by Winchester, B. G.

Search for Related Content

PubMed

PubMed Citation

Articles by Mills, K.

Articles by Winchester, B. G.

Related Collections

Molecular Diagnostics and Genetics

Proteomics and Protein Markers

Automation and Analytical Techniques