N-Acetylated Metabolites in Urine: Proton Nuclear Magnetic Resonance Spectroscopic Study on Patients with Inborn Errors of Metabolism

doi:10.1373/clinchem.2003.020214

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

Molecular Diagnostics and Genetics

N-Acetylated Metabolites in Urine: Proton Nuclear Magnetic Resonance Spectroscopic Study on Patients with Inborn Errors of Metabolism

Udo F.H. Engelke¹, Maria L.F. Liebrand-van Sambeek¹, Jan G.N. de Jong¹, Jules G. Leroy³, Éva Morava², Jan A.M. Smeitink² and Ron A. Wevers¹^,a

University Medical Center Nijmegen,¹ Laboratory of Pediatrics and Neurology and ² Department of Pediatrics, NL-6500 HB Nijmegen, The Netherlands.
³ Ghent University School of Medicine, Departments of Pediatrics and Medical Genetics, Ghent, Belgium.

^aAddress correspondence to this author at: University Medical Center Nijmegen, Laboratory of Pediatrics and Neurology (319), Institute of Neurology, Reinier Postlaan 4, 6525 GC Nijmegen, The Netherlands. Fax 31-24-3540297; e-mail r.wevers{at}cukz.umcn.nl.

Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Background: There is no comprehensive analytical technique toanalyze N-acetylated metabolites in urine. Many of these compoundsare involved in inborn errors of metabolism. In the presentstudy, we examined the potential of proton nuclear magneticresonance (¹H-NMR) spectroscopy as a tool to identify and quantifyN-acetylated metabolites in urine of patients with various inbornerrors of metabolism.

Methods: We performed ¹H-NMR spectroscopy on a 500 MHz spectrometer.Using a combination of one- and two-dimensional correlationspectroscopy (COSY) ¹H-NMR spectra, we were able to assign andquantify resonances of characteristic N-acetylated compoundsproducts in urine of patients with 13 inborn errors of metabolism.

Results: The disease-specific N-acetylated metabolites wereexcreted at concentrations >100 µmol/mmol of creatininein the patients’ urine. In control urine samples, theconcentration of individual N-acetyl-containing compounds was<40 µmol/mmol of creatinine. The combination of one-and two-dimensional COSY NMR spectroscopy led to the correctdiagnosis of nine different inborn errors of metabolism. Noabnormalities were observed in the spectra of urine from patientswith G_M1- or G_M2-gangliosidosis. We also determined the ¹H-NMRcharacteristics of N-acetylated metabolites that may be relevantto human metabolism.

Conclusion: ¹H-NMR spectroscopy may be used to identify andquantify N-acetylated metabolites of diagnostic importance forthe field of inborn errors of metabolism.

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Proton nuclear magnetic resonance (¹H-NMR) ¹ spectroscopy ofbody fluids has been used to diagnose inborn errors of metabolism(1)(2)(3). The technique yields an overview of proton-containingmetabolites, is rapid and nondestructive, and requires minimalsample pretreatment. In this report, we document the effectiveuse of ¹H-NMR spectroscopy for the identification and quantificationof N-acetyl-containing metabolites in body fluids of patientswith various inborn errors of metabolism. N-Acetylation occursin many metabolic pathways, which makes the detection of N-acetylatedcompounds important. Several diseases are known to be associatedwith the accumulation of N-acetylated metabolites. Some of thesehave been studied by ¹H-NMR spectroscopy. The urinary excretionof N-acetylated amino acids has been published for patientswith inborn errors of amino acid metabolism (4)(5). N-Acetylasparticacid and N-acetylaspartylglutamic acid are the laboratory markermetabolites in Canavan disease (6). Other authors have describedone- and two-dimensional NMR experiments for structural characterizationand identification of N-acetylneuraminic acid-containing storageproducts in lysosomal diseases (7)(8)(9). These studies demonstratethat the detection of N-acetylated metabolites assists in thediagnosis of various inborn errors of metabolism. However, manyN-acetylated compounds remain undetected by the conventionalanalytical techniques used in metabolic screening laboratories.

The three equivalent N-acetyl protons resonate as a singletin a small part of the ¹H-NMR spectrum (1.9–2.2 ppm).Only a few other metabolites are known to cause resonances inthis area. The finding of singlet signals in a one-dimensionalproton NMR spectrum can thus be used as an indication of thepresence of an N-acetylated metabolite.

We present here the NMR characteristics of many N-acetylatedcompounds relevant for human metabolism. In addition, we providesNMR spectra for urines representative for 13 inborn errors ofmetabolism that involve N-acetylated compounds.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

model compounds
Most model compounds were commercially available from Sigmaor Aldrich. N-Acetylated oligosaccharides from lysosomal storagediseases were isolated preparatively from thin-layer chromatography(TLC) plates routinely used for mono- and oligosaccharide analysisfrom urine of affected patients. Man ${alpha}$ 1-3Manß1-4-N-acetylglucosamine(GlcNAc), Fuc-GlcNAc-Asn, aspartylglucosamine, and two sialyloligosaccharideswere isolated with a butanol–acetic acid–water (2:1:1by volume) solvent system and visualized with orcinol–sulfuricacid (Fig. 1 ). Because of an overlap with lactose, Manß1-4GlcNAcfrom the urine of a ß-mannosidosis patient was isolatedwith propanol–acetic acid–water (42.5:0.5:7.5 byvolume) solvent system. The characteristic TLC bands were removedpreparatively from the silica-coated plate and measured as amodel compound.

View larger version (39K):
[in this window]
[in a new window]

Figure 1. Thin-layer chromatogram of dextran and urine samples.

The solvent system was butanol–acetic acid–water or orcinol–sulfuric acid. Lanes: 1, dextran; 2, sample from a patient with ${alpha}$ -mannosidosis; 3, sample from a patient with fucosidosis; 4, sample from a patient with G_M2-gangliosidosis; 5, sample from a patient with G_M1-gangliosidosis; 6, dextran; 7, sample from a healthy individual; 8, sample from a patient with aspartylglucosaminuria; 9, sample from a patient with sialidosis. The arrows indicate the characteristic TLC bands.

urine
Control urine samples were from 10 healthy individuals and from50 diseased patients. In the urine samples from diseased controlssent to our laboratory, extensive metabolic screening had ruledout any relevant inborn errors of metabolism.

Urine was centrifuged before analysis. We added 70 µLof a 20.2 mmol/L trimethylsilyl-2,2,3,3-tetradeuteropropionicacid (sodium salt; Aldrich) ²H₂O solution to 700 µL ofurine as a chemical shift reference ( ${delta}$ = 0.00) and as a locksignal. The pH of the urine was adjusted to 2.50 ± 0.05with concentrated HCl. Finally, we placed 650 µL of thesample in a 5-mm NMR tube (Wilmad Royal Imperial).

nmr measurements
High-resolution spectra for urine samples and the model compoundswere acquired at 500 MHz on a Bruker DRX and AMX spectrometerequipped with a sample changer.

The spin-lattice or longitudinal relaxation time (T₁) valuesfor N-acetylneuraminic acid, N-aspartylglucosamine, N-acetylasparticacid, and Man(1-4)GlcNAc, as representative N-acetylated compounds,were determined in urine of patients by the inversion-recoverytechnique. The T₁ values amounted to 1.0, 0.9, 1.6, and 0.9s, respectively.

one-dimensional ¹h-nmr spectroscopy
For urine, 128 transients were collected into 32 000 data pointswith a spectral width of 6002 Hz. The H₂O resonance was presaturatedduring the relaxation delay (10 s). Shimming of the sample wasperformed automatically on the deuterium signal.

A sine-bell squared filter (SSB = 2) was used, and spectra wereFourier-transformed after the free induction decay was zero-filledto 64 000 data points. The phase and the baseline were correctedmanually. The N-acetyl resonances in the one-dimensional urinespectra were fitted semiautomatically to a Lorentzian line shapemodel function. The integrals of these fits were used for quantificationby comparing them to the fit integral of creatinine (singletat 3.13 ppm). For identification and quantification of the NMRspectra, 1D WinNMR and the AMIX software were used (Bruker BioSpin).A prerequisite for accurate quantitative determination of metaboliteswith proton NMR spectroscopy lies in the length of the relaxationdelay. We used a delay of 10 s, which is more than five timesthe T₁ value of the N-acetyl protons in N-acetylaspartic acid,the compound with the longest T₁ value among the N-acetylatedcompounds.

¹h-¹h correlation spectroscopy (cosy)
The spectral widths in the F₁ and F₂ axes were 6002 Hz, and4000 data points were collected in F₂. For the urine samples,256 increments and 16 scans per increment were used. The relaxationdelay was 2 s, and before the Fourier transformation, a sinefunction was applied in both time domains. During the relaxationdelay, the water resonance was presaturated.

quantitative data
To study the linearity and recovery, we added three N-acetylatedmetabolites, N-acetyltyrosine (cat. no. A-2513; Sigma), N-acetyltryptophan(cat. no. A-6376; Sigma), and N-acetylaspartic acid (cat. no.A-5625; Sigma), separately to normal human urine in concentrationsof 0, 100, 500, and 3000 µmol/L. After addition of thesemetabolites the creatinine concentration of the urine was 1.1mmol/L. The same experiment was repeated with a second urinewith a creatinine concentration of 2.0 mmol/L. For concentrationcalculations for the N-acetylated metabolites using ¹H-NMR spectroscopy,we used trimethylsilyl-2,2,3,3-tetradeuteropropionic acid asthe concentration reference, and the metabolite concentrationswere expressed in µmol/L.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

n-acetyl resonances in urine
A representative ¹H-NMR spectrum of urine from a healthy individualis shown in Fig. 2 . Methyl protons from N-acetyl groups characteristicallygive a singlet resonance in a limited part of the ¹H-NMR spectrum(1.9–2.2 ppm). Table 1 provides an overview of the N-acetyl-containingmetabolites detectable in urine samples from healthy individualsand patients. Individual compounds can be recognized by thechemical shift of the N-acetyl group CH₃ protons and from resonancesderiving from other parts of the molecule. Neuraminic acid,N-acetylaspartic acid, and the N-acetyl groups in glycoproteinsin urine from healthy controls are known to contribute to theresonances in this area (10). In addition, a few metaboliteswithout an N-acetyl group are known to resonate between 1.9and 2.2 ppm. These include glutamine (ß-CH₂ multipletat 2.15 ppm), proline (ß-CH₂ multiplet at 2.02 ppm),methionine (S-CH₃ singlet at 2.13 ppm) (11), and acetic acid(CH₃ singlet at 2.08 ppm).

View larger version (18K):
[in this window]
[in a new window]

Figure 2. 500 MHz ¹H-NMR spectrum of urine from a healthy volunteer.

The creatinine peak (singlet at 3.13 ppm) is scaled to 100. The inset show the N-acetyl region in greater detail.

View this table:
[in this window]
[in a new window]

Table 1. ¹H resonance positions and multiplicity of N-acetyl-containing metabolites.

quantitative data
The linearity was excellent for all three N-acetylated metabolites,N-acetyltyrosine, N-acetyltryptophan, and N-acetylaspartic acid(slope, 0.94–1.09; intercept did not significantly deviatefrom zero; correlation coefficient >0.99). The recovery wasin 90–110% for these compounds at all concentrations.

To study the reproducibility (within-run), we prepared and measured10 samples from the same urine on the same day. The within-runCV at 3000 µmol/L was <4% for all three N-acetylatedmetabolites.

strategy for quantitative interpretation and assignment
Because of the low concentrations of N-acetylated metabolites,assignment of their singlet resonances in urine from healthyvolunteers is generally not possible. Metabolic diseases thatinvolve N-acetylated compounds may be diagnosed if the concentrationsof the characteristic N-acetylated metabolites are high enoughto qualify them as abnormal and to allow their identification.Identification requires the spectral information from the protonsin the rest of the molecule (Table 1 ). As a systematic approach,we quantified the highest singlet resonance between 1.9 and2.2 ppm. Excluded from this quantification was the singlet foracetic acid (mean chemical shift, 2.083 ppm; minimum, 2.081ppm; maximum, 2.085 ppm; n = 10). It was assumed that CH₃ protonsfrom N-acetylated metabolites cause the resonances in this region.Fig. 3 shows the concentrations of individual N-acetyl-containingcompounds in urine samples from 50 diseased controls and 10healthy volunteers. The highest concentration of an N-acetylatedcompound was generally <40 µmol/mmol of creatinine.Higher concentrations were observed in children under 5 years.Especially in the first month of life, values up to 200 µmol/mmolof creatinine could be found. Fig. 3 also shows data on urinesamples from patients with 13 different inborn errors of metabolisminvolving N-acetylated compounds. Below 40 µmol/mmol ofcreatinine, the CH₃ protons from the N-acetyl group are theonly resonances from most N-acetylated compounds that can beobserved in the spectra. Therefore, assignments based solelyon the N-acetyl singlet were not possible. As shown in Fig.3 , most patients with inborn errors of metabolism excretedthe N-acetylated metabolites typical for their diseases at concentrations>100 µmol/mmol of creatinine. At such concentrations,the typical N-acetyl compound could be assigned with greatercertainty because the other protons of the molecule contributeto the assignment. Two-dimensional COSY spectra may help withfurther identification of relevant metabolites. As an example,Fig. 4 shows how specific cross-peaks in a two-dimensionalCOSY spectrum of the model compound Fuc-GlcNAc-Asn (Fig. 4A )can help to identify this metabolite in the urine of a patientwith fucosidosis (Fig. 4B ). The cross-peaks derive from theGlcNAc protons (3.83–5.10 and 3.78–4.90 ppm), theAsn protons (2.94–4.06 ppm), and the Fuc protons (1.21–4.12ppm).

View larger version (9K):
[in this window]
[in a new window]

Figure 3. Quantification of the N-acetylated compound with the highest concentration in the urine as function of age.

${circ}$ , controls; •, urine of affected patients. 1, Salla disease; 2, French-type sialuria; 3, ${alpha}$ -mannosidosis; 4, ß-mannosidosis; 5, fucosidosis; 6, aspartylglucosaminuria; 7, G_M1-gangliosidosis; 8, G_M2-gangliosidosis; 9, sialidosis; 10, Canavan disease; 11, citrullinemia; 12, tyrosinemia type I; 13, tyrosinemia type II.

View larger version (22K):
[in this window]
[in a new window]

Figure 4. COSY spectra of model compound Fuc-GlcNAc-Asn obtained from TLC chromatography (A) and urine from a patient with fucosidosis (B).

The characteristic pattern of the model compound Fuc-GlcNAc-Asn is shown in the circled cross-peaks.

inborn errors of metabolism
Infantile sialic acid storage disorder (ISSD; OMIM 269920)/Salla disease (OMIM 604369).
ISSD and Salla disease are both characterized by increased concentrationsof free sialic acid (N-acetylneuraminic acid) in the urine andby its storage in the lysosomes of different tissues. The molecularbasis of these diseases is a defect in the lysosomal sialicacid transporter. Severe mutations in the gene lead to ISSD,whereas milder mutations clinically present as Salla disease.Characteristically, a 20- to 200-fold increase in N-acetylneuraminicacid excretion in urine has been described in infantile casesof the disease. Bound sialic acid typically is within the rangeobtained for controls.

One- and two-dimensional COSY ¹H-NMR spectra were obtained fromurine of a 16-year-old patient with Salla disease. The one-dimensionalurine spectrum showed the presence of N-acetylneuraminic acid[singlet at 2.05 ppm; 121 µmol/mmol of creatinine; referencevalues, 20.2 (11.6) µmol/mmol of creatinine for ages >2years (12); Fig. 5A ]. The COSY spectrum confirmed the presenceof free N-acetylneuraminic acid by showing cross-peaks fromthe pyranose ring protons of the carbon-3 atom (1.85 and 2.26ppm; data not shown) (13).

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

Figure 5. 500 MHz ¹H-NMR spectra of urine samples.

(A), Salla disease; (B), French-type sialuria; (C), ${alpha}$ -mannosidosis; (D), ß-mannosidosis; (E), fucosidosis; (F), aspartylglucosaminuria; (G), G_M1-gangliosidosis; (H), G_M2-gangliosidosis; (I), sialidosis; (J), Canavan disease; (K), citrullinemia; (L), tyrosinemia type I. The creatinine peak (singlet at 3.13 ppm; not shown) in the urine spectra is scaled to 100.

French-type sialuria (OMIM 269921).
French-type sialuria is a metabolic disorder caused by a defectthe enzyme uridine diphosphate-N-acetylglucosamine 2-epimerase(EC 5.1.3.14), which is involved in N-acetylneuraminic acidsynthesis. The defect in the enzyme leads to failing feedbackinhibition by N-acetylneuraminic. Free N-acetylneuraminic acidis massively increased in the body fluids of diseased patients.We investigated the urine of a 6-year-old child with this disease.N-Acetylneuraminic acid excretion (Fig. 5B ) was much higherthan in the patient with Salla disease [4275 µmol/mmolof creatinine; reference values, 20.2 (11.6) µmol/mmolof creatinine for ages >2 years (12)].

Because of the very high concentration of N-acetylneuraminicacid, even the pyranose ring protons (3.5–4.1 ppm) andthe nitrogen proton (doublet at 8.09 ppm) were clearly observedin the one- and two-dimensional spectra (data not shown).

${alpha}$ -Mannosidosis (OMIM 248500).
Patients with a deficiency of the lysosomal enzyme ${alpha}$ -mannosidase(EC 3.2.1.24) have high concentrations of Man_nGlcNAc (n $>=$ 2)oligosaccharides in the cells and urine.

Oligosaccharide TLC of the urine from an affected patient showedmany mannose-rich oligosaccharide bands. The major oligosaccharideband (Fig. 1 , lane 2) typical for this defect was isolatedpreparatively from the silica-coated plate and measured as amodel compound by ¹H-NMR. The compound was identified by comparisonwith reference spectra as the trisaccharide Man ${alpha}$ 1-3Manß1-4GlcNAc(14).

One- and two-dimensional COSY ¹H-NMR spectra were obtained fromurine of the patient. In the COSY spectrum, Man ${alpha}$ 1-3Manß1-4GlcNAcwas recognizable as two cross-peaks (4.04–5.10 and 3.88–5.20ppm), and in the one-dimensional spectrum was recognizable asa singlet at 2.03 ppm (Fig. 5C ) and doublet at 5.20 ppm. Theurinary concentration of Man ${alpha}$ 1-3Manß1-4GlcNAc in ourpatient was 153 µmol/mmol of creatinine.

ß-Mannosidosis (OMIM 248510).
The lysosomal enzyme ß-mannosidase is involved inglycoprotein catabolism. A deficiency of this enzyme leads toexcessive urinary excretion of the disaccharide Manß1-4GlcNAc.

We measured urine samples from two brothers (ages 8 and 9 years)with ß-mannosidosis. Oligosaccharide TLC was performedon urine samples from the boys. The Manß1-4GlcNAcband (data not shown) was isolated preparatively from the silica-coatedplate (100 µg) and measured as a model compound by ¹H-NMR.The spectrum showed the N-acetyl singlet (2.03 ppm), the 1 ${alpha}$ and1ß GlcNAc protons (doublets at 4.72 and 5.20 ppm,respectively), and many resonances in the 3.4–4.1 regionderiving from the GlcNAc and Man parts of the disaccharide.The one-dimensional NMR spectra of their urine showed the samesinglets at 2.04 ppm (Fig. 5D ) and doublets at 5.21 ppm. Thedoublet at 4.72 ppm was not visible because of overlap of thewater resonance. The COSY spectra from the urine showed characteristiccross-peaks from the 1 ${alpha}$ and 1ß GlcNAc protons (3.89–5.20and 3.72–4.72 ppm, respectively; data not shown). TheManß1-4GlcNAc concentrations in the urine of the brotherswere 255 and 273 µmol/mmol of creatinine. Another, smallersinglet at 2.03 ppm was also observed in the one-dimensionalNMR spectra of the two brothers (56 and 122 µmol/mmolof creatinine). Presumably this compound is sialyl- ${alpha}$ 2-6-mannosyl-ß1-4-N-acetylglucosamine( $~$ 10% of the concentration of Manß1-4GlcNAc). Van Peltet al. have identified this trisaccharide in concentrated urinefractions of affected patients (7).

Fucosidosis (OMIM 230000).
Because of a deficiency of lysosomal ${alpha}$ -L-fucosidase (EC 3.2.1.51),patients with fucosidosis accumulate fucose-containing glycolipids,oligosaccharides, or glycoasparagines in the urine and tissue.Three characteristic oligosaccharides were isolated from urineof an affected patient by TLC (Fig. 1 , lane 3). These bandswere removed from the TLC plate and dissolved in ²H₂O. The fractionswere analyzed by ¹H-NMR spectroscopy and compared with the literature(15). The one- and two-dimensional spectra of fraction 1 indicatedthe presence of Fuc-GlcNAc-Asn (Table 1 ). Because of the lowconcentrations in the isolated fractions 2 and 3, interpretationwas impossible.

The characteristic COSY pattern of Fuc-GlcNAc-Asn (cross-peaksat 1.21–4.12 and 2.94–4.06 ppm) was observed inthe spectrum for urine from an affected adult patient (Fig.4B ). The urinary Fuc-GlcNAc-Asn concentration was 109 µmol/mmolof creatinine (singlet at 2.01 ppm; Fig. 5E ).

Aspartylglucosaminuria (OMIM 208400).
Aspartylglucosaminidase deficiency or aspartylglucosaminuriais an inborn error of metabolism caused by the deficiency ofthe lysosomal enzyme N-aspartyl-ß-glucosylaminidase(EC 3.5.1.26). This enzyme cleaves the N-acetylglucosamine–asparaginelinkage found in a variety of oligosaccharides and glycoproteins.Patients with the disease excrete aspartylglucosamine (GlcNAc-Asn)as major abnormal metabolite. In addition, several other glycoasparagines,such as Galß1-4GlcNAcß1-N-Asn, the mannose-richderivative Man-Man-GlcNAc-GlcNAc-Asn, and NeuAc-Gal-GlcNAc-Asn,can be excreted (16). Urine samples from two unrelated caseswere available. TLC with orcinol–sulfuric acid showedthe abnormal Galß1-4GlcNAcß1-N-Asn bandin these samples (Fig. 1 , lane 9). TLC plates stained withninhydrin showed the GlcNAc-Asn and the Galß1-4GlcNAcß1-N-Asnband in the urine (data not shown). The NMR spectra of nearlypure compounds were compared with reference spectra from theliterature (17). The resonances of both compounds are shownin Table 1 . The characteristic cross-peaks of both compoundswere observed in COSY spectra of urine from both patients. TheGlcNAc-Asn concentrations (singlet at 2.02 ppm; Fig. 5F ) were169 and 323 µmol/mmol of creatinine, respectively. TheGalß1-4GlcNAcß1-N-Asn (singlet at 2.01 ppm)concentrations were 27 (case 1) and 114 µmol/mmol of creatinine(case 2).

G_M1-Gangliosidosis (OMIM 230500).
A deficiency of ß-D-galactosidase (EC 3.2.1.23) leadsto G_M1-gangliosidosis. Oligosaccharides with a D-galactosylgroup at the nonreducing end are increased in the urine of affectedpatients.

Three bands were isolated preparatively by TLC from the urineof an affected patient (Fig. 1 , lane 5) and compared with spectrafrom the literature (17). The NMR spectrum of band 2 correspondedto the biantennary octasaccharide (17), and the NMR spectrumof band 3 corresponded to the triantennary decasaccharide (17)or the tetraantennary dodecasaccharide (17). For band 1, wecould not find an exact match with reference spectra.

The one-dimensional NMR spectrum of urine from an affected patient(Fig. 5G ) showed singlets between 2.00 and 2.04 ppm. The singletwith the highest intensity (2.03 ppm) represented a N-acetylatedstorage compound with a concentration of 34 µmol/mmolof creatinine.

G_M2-Gangliosidosis (Sandhoff disease; OMIM 268800).
As a result of a deficiency in ß-N-acetylhexosaminidase(EC 3.2.1.52), oligosaccharides containing N-acetylglucosamineare excreted in the urine of affected patients.

Using TLC, we were able to preparatively isolate two bands fromthe urine of an affected patient (Fig. 1 , lane 4). The NMRspectra of both isolated bands showed resonances at 5.20, 5.11,and 4.53 and a singlet at 2.05 ppm. Band 2 differed from band1 by an additional doublet at 4.46 ppm and two more singlets(2.045 and 2.06 ppm). The chemical shift data point to oligosaccharideswith the structures ß-GlcNAc-(1 $->$ 2)- ${alpha}$ -Man-(1-3)-[ß-GlcNAc-(1 $->$ 2)- ${alpha}$ -Man-(1-6)]-ß-Man-(1 $->$ 4)-GlcNAcfor band 1 and ß-GlcNAc-(1 $->$ 2)- ${alpha}$ -Man-(1-3)-[ß-GlcNAc-(1 $->$ 4)][ß-GlcNAc-(1 $->$ 2)]- ${alpha}$ -Man-(1-6)]-ß-Man-(1 $->$ 4)-GlcNAcfor band 2 (18).

The one-dimensional NMR spectrum for urine of an affected patient(Fig. 5H ) showed singlets between 2.02 and 2.08 ppm. The singletwith the highest intensity (2.06 ppm) represents a N-acetylatedstorage compound at a concentration of 77 µmol/mmol ofcreatinine.

Sialidosis (OMIM 256550).
Sialidosis, or mucolipidosis I, is caused by a deficiency ofthe lysosomal enzyme neuraminidase. The enzyme cleaves terminal ${alpha}$ 2 $->$ 3 and ${alpha}$ 2 $->$ 6 sialyl linkages of various glycopeptides, oligosaccharides,and gangliosides. High concentrations of sialyloligosaccharides(bound sialic acid) are found in urine of affected patients.

At least six singlet resonances with a concentration >50µmol/mmol of creatinine were found between 2.0 and 2.1ppm by one-dimensional ¹H-NMR spectroscopic analysis of theurine of our patient (Fig. 5I ). The COSY spectrum of the urineshowed two cross-peaks: 1.72–2.67 ppm from the ${alpha}$ 2 $->$ 6 sialyllinkages and 1.81–2.67 ppm from the ${alpha}$ 2 $->$ 3 sialyl linkages(data not shown). The singlet with the highest intensity (2.03ppm) was present at a concentration of 430 µmol/mmol ofcreatinine.

Using TLC, we preparatively isolated two oligosaccharides fromthe urine of an affected patient (Fig. 1 , lane 9). We observedtwo multiplets (1.75 and 2.66 ppm; cross-peak in the COSY spectrum)in the NMR spectra of both isolated compounds. This allowedus to conclude that both isolated compounds have an ${alpha}$ 2 $->$ 6 sialyllinkage. In the spectrum for band 1, three N-acetyl singletsresonated at 2.02, 2.03, and 2.06 ppm, deriving from the twoGlcNAc units and the acetylneuraminic acid (NeuAc) unit. Fromits spectrum we could conclude that band 1 probably is ${alpha}$ -NeuAc-(2 $->$ 6)-ß-Gal-(1 $->$ 4)-ß-GlcNAc-(1 $->$ 2)- ${alpha}$ -Man-(1 $->$ 3)-ß-Man-(1 $->$ 4)-GlcNAc(19).

Band 2 differed in the chemical shift position of one acetylsinglet (2.05 instead of 2.03 ppm) and the presence of an additionalsignal at 4.11 ppm, which could indicate compound V in the reportby Dorland et al. (19).

Canavan disease (OMIM 271900).
Canavan disease is a leukodystrophy attributable to a deficiencyof aspartoacylase (EC 3.5.1.15) and belongs to the group ofneurotransmitter diseases. We analyzed urine from two unrelatedpatients. The one-dimensional ¹H-NMR spectra for body fluidshowed the presence of high concentrations of N-acetylasparticacid [Fig. 5J ; urine from case A, 1760 µmol/mmol of creatinine;urine from case B, 1474 µmol/mmol of creatinine; referencevalues for all ages, 6–36 µmol/mmol of creatinine(20)].

Citrullinemia (OMIM 215700).
Deficiency of the urea cycle enzyme argininosuccinate synthase(EC 6.3.4.5) leads to increased concentrations of citrullineand N-acetylcitrulline in the urine (4)(21).

We analyzed two urine samples from a patient with citrullinemia.The urine ¹H-NMR spectrum showed citrulline multiplets (concentration,825 µmol/mmol of creatinine). We assigned the unusuallyhigh singlet at 2.03 ppm to N-acetylcitrulline by comparingthe chemical shifts with reference spectra in the literature(22). N-Acetylcitrulline is not commercially available. Theurinary N-acetylcitrulline concentrations were 441 and 518 µmol/mmolof creatinine (Fig. 5K ).

Tyrosinemia type I (OMIM 276700).
Tyrosinemia type I is caused by a deficiency of the enzyme fumarylacetoacetatehydrolase (EC 3.7.1.2). High body fluid concentrations of tyrosine,4-hydroxyphenylacetic acid, 4-hydroxyphenyllactic acid, succinylacetone,and methionine are characteristic of affected patients. We analyzedthe urine of a 1-year-old boy with this inborn error.

In one-dimensional ¹H-NMR spectra of his urine, we observedhigh concentrations of tyrosine and 4-hydroxyphenyllactic acid;the concentrations of betaine and methionine were also high.In addition to these typical tyrosinemia type 1 metabolites,we found a high concentration of N-acetyltyrosine (singlet at1.94 ppm; 195 µmol/mmol of creatinine; Fig. 5L ). We identifiedthe compound by comparing the spectrum with the model compound(singlet at 1.94 ppm; AB system at 3.07 ppm and AB system at7.89 ppm). Succinylacetone and succinylacetoacetate, the biochemicalhallmarks in tyrosinemia type I, could not be demonstrated byNMR spectroscopy in this urine.

Tyrosinemia type II (OMIM 276600).
Deficiency of the cytosolic enzyme tyrosine aminotransferase(EC 2.6.1.5) forms the primary defect of tyrosinemia type II.In the liver it leads to high concentrations of tyrosine, 4-hydroxyphenyllacticacid, 4-hydroxyphenylacetic acid, 4-hydroxyphenylpyruvic acid,and N-acetyltyrosine in body fluids. Urine from one patientwas analyzed. The concentration of N-acetyltyrosine in the urineof an affected patients was 95 µmol/mmol of creatinine(singlet at 1.94 ppm).

In another patient (age, 0.2 years), we observed a much higherconcentration of N-acetyltyrosine in the urine (>3000 µmol/mmolof creatinine). This patient received parenteral nutrition containingN-acetyltyrosine. In premature infants (gestational age at birth<36 weeks), urinary N-acetyltyrosine may be as high as 781µmol/mmol of creatinine (23). In addition, N-acetyltyrosinemay be increased in some liver diseases, in which it may beobserved along with N-acetyltryptophan (Table 1 ).

Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

N-Acetylated compounds are metabolites in many metabolic pathwaysand therefore may relate to various inborn errors of metabolism.In this study, we gave examples of 13 inherited diseases involvingN-acetylated metabolites. At present, a comprehensive analyticaltechnique to detect and identify N-acetylated compounds in bodyfluids is not available. However, N-acetylaspartic acid, thebiochemical hallmark in Canavan disease, is detected by organicacid analysis by gas chromatography–mass spectrometry.Gas chromatography–mass spectrometry can also be usedfor the accurate diagnosis of tyrosinemia by analysis for allrelevant metabolites, including N-acetyltyrosine. TLC is usefulin the identification of abnormal N-acetylated oligosaccharidescharacteristic of some of the lysosomal storage disorders.

NMR spectroscopy of body fluids can provide an overview of N-acetylatedcompounds. The protons of the N-acetyl group resonate in a specificnarrow region of the spectrum. For metabolic screening purposes,we used the highest resonance in the N-acetyl region to identifysamples with unusually high concentrations of an N-acetylatedmetabolite (Fig. 3 ). This approach allowed different N-acetylatedmetabolites to be quantified in individual samples. For example,in the urine of a young child, the singlet at 1.94 ppm gavethe highest concentration, whereas in an adult urine, the highestconcentration was for the singlet at 2.04 ppm. As shown in Fig.3 , most patients with inborn errors of metabolism excretedthe N-acetylated metabolites typical for their diseases at concentrations>100 µmol/mmol of creatinine. In 10 of the 13 inbornerrors of metabolism, this concentration was clearly higherthan the upper limit of the reference interval. In all of thesecases the combination of one-dimensional spectroscopy and COSYspectra allowed identification of the compound of interest.This led to the correct diagnosis in 9 of the 13 cases. Exceptionsincluded the urines from patients with tyrosinemia type I andII and G_M1- and G_M2-gangliosidosis.

In tyrosinemia type I, the excretion of succinylacetone andsuccinylacetoacetate in urine is the diagnostic hallmark. Todate, gas chromatography–mass spectrometry remains themethod of choice to determine succinylacetone and the othercharacteristic metabolites and to diagnose tyrosinemia typeI. For similar reasons the same holds true for tyrosinemia typeII.

Because of the relatively low urinary concentrations of theG_M1- and G_M2-gangliosidosis metabolites (34 and 77 µmol/mmolof creatinine), assignment of these metabolites in urine inaffected patients was not possible, and the diagnosis of G_M1-and G_M2-gangliosidosis was missed by ¹H-NMR. NMR spectrometerswith higher fields (>500 MHz) and spectrometers using theincreased sensitivity of CryoProbe technology could probablydetect these two inborn errors of metabolism.

In spite of pH standardization, assignments of structure basedsolely on the chemical shift of the N-acetyl protons are insufficientbecause many acetyl singlets may occur in urine. Therefore,characteristic COSY patterns of model compounds are requiredto confirm the presence of individual N-acetylated metabolitesin a patient’s urine. For example, the acetyl protonsof N-acetylaspartic acid and Man(1-4)GlcNAc showed a singletat the same chemical shift (2.03 ppm) in the one-dimensionalspectrum. Two-dimensional COSY NMR experiments showed for eachmodel compound different and characteristic cross-peaks producedby protons elsewhere in the molecule (Table 1 ). Because ofa change in structure, bound N-acetylneuraminic acid can bedistinguished from free N-acetylneuraminic acid in two-dimensionalCOSY ¹H-NMR spectra (Table 1 ). This makes it possible to differentiatepatients with isolated neuraminidase deficiency, who excretebound N-acetylneuraminic acid, from patients with Salla diseaseor French type sialuria, who excrete excess free N-acetylneuraminicacid in urine (13). However, in regions with a high densityof resonances, especially around the two-dimensional COSY diagonal,cross-peaks sometimes show overlap and cannot be used for correctassignments. Other two-dimensional NMR techniques, such as J-resolvedspectroscopy and total correlation spectroscopy, can be usedto help with further interpretation.

The use of medications can be a pitfall in the quantificationof N-acetylated metabolites. The antiepileptic drug Sabril®(vigabatrin) is often used in patients suspected to have aninborn error of metabolism. The H-NMR urine spectra of Sabril-treatedpatients show high Sabril resonances between 2.0 and 2.1 ppmcaused by CH₂ protons (multiplet). This Sabril multiplet interfereswith the N-acetyl resonances. Therefore, correct interpretationand quantification of the N-acetyl region of the H-NMR spectrumis impossible. Some drugs can be converted in the body to theiracetylated conjugates. Acetaminophen, for example, is metabolizedin the body and is excreted in the urine in various forms. The¹H-NMR spectrum of urine may show acetaminophen (paracetamol;singlet at 2.14 ppm), 4-glucuronosidoacetanilide (singlet at2.15 ppm), N-acetyl-4-aminophenol sulfate (singlet at 2.17 ppm),and N-acetyl-2-(N-acetyl-L-cysteinyl)-4-aminophenol (24).

In conclusion, we have shown that careful inspection and quantitativeinterpretation of the N-acetyl region of the ¹H-NMR spectrummay identify an abnormally high concentration of an N-acetylatedmetabolite. The technique is uniquely suited for studying patientswith inborn errors of metabolism, and our data extend that todiseases involving N-acetylated metabolites. A combination ofone- and two-dimensional COSY ¹H-NMR spectroscopy identifiedat least nine different inborn errors of metabolism involvingN-acetylated metabolites.

Acknowledgments

The ¹H-NMR spectra were recorded at the Dutch hf-NMR facilityat the Department of Biophysical Chemistry, University of Nijmegen,The Netherlands (Prof. Sybren Wijmenga, department head). Wethank Jos Joordens for invaluable help and technical assistance.We also thank Drs. Neidig and Fischer (Bruker BioSpin, Karlsruhe,Germany) for invaluable help and improvements in the AMIX software.

Footnotes

Previously published online at DOI: 10.1373/clinchem.2003.020214

¹ Nonstandard abbreviations: ¹H-NMR, proton nuclear magnetic resonance;TLC, thin-layer chromatography; GlcNAc, N-acetylglucosamine;COSY, correlation spectroscopy; and ISSD, infantile sialic acidstorage disorder.

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Iles RA, Hind AJ, Chalmers RA. Use of proton nuclear magnetic resonance spectroscopy in detection and study of organic acidurias. Clin Chem 1985;31:1795-1801.[Abstract/Free Full Text]
Wevers RA, Engelke U, Heerschap A. High-resolution ¹H-NMR spectroscopy of blood plasma for metabolic studies. Clin Chem 1994;40:1245-1250.[Abstract/Free Full Text]
Wevers RA, Engelke U, Wendel U, de-Jong JG, Gabreels FJ, Heerschap A. Standardized method for high-resolution ¹H-NMR of cerebrospinal fluid. Clin Chem 1995;41:744-751.[Abstract/Free Full Text]
Strandholm JJ, Buist NR, Kennaway NG, Curtis HT. Excretion of ${alpha}$ -N-acetylcitrulline in citrullinaemia. Biochim Biophys Acta 1971;244:214-216.[Medline] [Order article via Infotrieve]
Jellum E, Horn L, Thoresen O, Kvittingen EA, Stokke O. Urinary excretion of N-acetyl amino acids in patients with some inborn errors of amino acid metabolism. Scand J Clin Lab Invest Suppl 1986;184:21-26.[Medline] [Order article via Infotrieve]
Burlina AP, Ferrari V, Divry P, Gradowska W, Jakobs C, Bennett MJ, et al. N-Acetylaspartylglutamate in Canavan disease: an adverse effector?. Eur J Pediatr 1999;158:406-409.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
van Pelt J, Dorland L, Duran M, Hokke CH, Kamerling JP, Vliegenthart JF. Sialyl- ${alpha}$ 2-6-mannosyl-ß1-4-N-acetylglucosamine, a novel compound occurring in urine of patients with ß-mannosidosis. J Biol Chem 1990;265:19685-19689.[Abstract/Free Full Text]
van Pelt J, Hard K, Kamerling JP, Vliegenthart JF, Reuser AJ, Galjaard H. Isolation and structural characterization of twenty-one sialyloligosaccharides from galactosialidosis urine. An intact N,N'-diacetylchitobiose unit at the reducing end of a diantennary structure. Biol Chem Hoppe Seyler 1989;370:191-203.[Web of Science][Medline] [Order article via Infotrieve]
van Pelt J, Kamerling JP, Bakker HD, Vliegenthart JF. A comparative study of sialyloligosaccharides isolated from sialidosis and galactosialidosis urine. J Inherit Metab Dis 1991;14:730-740.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
Lindon JC, Nicholson JK, Everett JR. NMR spectroscopy of biofluids. Annu Rep NMR Spectrosc 1999;38:1-88.
Parvy PR, Bardet JI, Rabier DM, Kamoun PP. Age-related reference values for free amino acids in first morning urine specimens. Clin Chem 1988;34:2092-2095.[Abstract/Free Full Text]
Romppanen J, Mononen I. Age-related reference values for urinary excretion of sialic acid and deoxysialic acid: application to diagnosis of storage disorders of free sialic acid. Clin Chem 1995;41:544-547.[Abstract/Free Full Text]
Sewell AC, Murphy HC, Iles RA. Proton nuclear magnetic resonance spectroscopic detection of sialic acid storage disease. Clin Chem 2002;48:357-359.[Free Full Text]
Hard K, Mekking A, Kamerling JP, Dacremont GA, Vliegenthart JF. Different oligosaccharides accumulate in the brain and urine of a cat with ${alpha}$ -mannosidosis: structure determination of five brain-derived and seventeen urinary oligosaccharides. Glycoconj J 1991;8:17-28.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
Michalski JC, Wieruszeski JM, Alonso C, Cache P, Montreuil J, Strecker G. Characterization and 400-MHz ¹H-NMR analysis of urinary fucosyl glycoasparagines in fucosidosis. Eur J Biochem 1991;201:439-458.[Web of Science][Medline] [Order article via Infotrieve]
Aula P, Jalanko A, Peltonen L. Aspartylglucosaminuria. Scriver CR Beaudet AL Valle D Sly WS eds. The metabolic and molecular bases of inherited diseases, 8th ed 2001:3535-3550 . .
. Biocarb Chemicals. Catalog with H-NMR spectra 1990 Biocarb Chemicals Lund, Sweden. .
Strecker G, Herlant-Peers MC, Fournet B, Montreul J. Structure of seven oligosaccharides excreted in the urine of a patient with Sandhoff’s disease (GM2 gangliosidosis-variant O). Eur J Biochem 1977;81:165-171.[Web of Science][Medline] [Order article via Infotrieve]
Dorland L, Haverkamp J, Viliegenthart JF, Strecker G, Michalski JC, Fournet B, et al. 360-MHz ¹H nuclear-magnetic-resonance spectroscopy of sialyl-oligosaccharides from patients with sialidosis (mucolipidosis I and II). Eur J Biochem 1978;87:323-329.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
Jakobs C, Verhoeven NM, van-der-Knaap MS. Various organic acidurias. Blau N Duran M Blaskovics ME Gibson KM eds. Physician’s guide to the laboratory diagnosis of metabolic diseases, 2nd ed 2002:225-226 Springer-Verlag Berlin. .
Ruitenbeek W, Kobayashi K, Iijima M, Smeitink JA, Engelke UF, De Abreu RA, et al. Moderate citrullinaemia without hyperammonaemia in a child with mutated and deficient argininosuccinate synthetase. Ann Clin Biochem 2003;40:102-107.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
Burns SP, Woolf DA, Leonard JV, Iles RA. Investigation of urea cycle enzyme disorders by ¹H-NMR spectroscopy. Clin Chim Acta 1992;209:47-60.[CrossRef][Web of Science][Medline] [Order article via Infotrieve]
Blau N Duran M Blaskovics ME Gibson KM eds. Physician’s guide to the laboratory diagnosis of metabolic diseases, 2nd ed 2002:38-39 Springer-Verlag Berlin. .
Spraul M, Hofmann M, Lindon JC, Farrant RD, Seddon MJ, Nicholson JK, et al. Evaluation of liquid chromatography coupled with high-field ¹H NMR spectroscopy for drug metabolite detection and characterization: the identification of paracetamol metabolites in urine and bile. NMR Biomed 1994;7:295-303.[Web of Science][Medline] [Order article via Infotrieve]

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

S. B. Wortmann, R. J. T. Rodenburg, A. Jonckheere, M. C. de Vries, M. Huizing, K. Heldt, L. P. van den Heuvel, U. Wendel, L. A. Kluijtmans, U. F. Engelke, et al.
Biochemical and genetic analysis of 3-methylglutaconic aciduria type IV: a diagnostic strategy
Brain, January 1, 2009; 132(1): 136 - 146.
[Abstract] [Full Text] [PDF]

N. Shanaiah, M. A. Desilva, G. A. Nagana Gowda, M. A. Raftery, B. E. Hainline, and D. Raftery
Class selection of amino acid metabolites in body fluids using chemical derivatization and their enhanced 13C NMR
PNAS, July 10, 2007; 104(28): 11540 - 11544.
[Abstract] [Full Text] [PDF]

J. Hunt
If It Smells Like a Duck, It Might Be an Asthma Subphenotype
Am. J. Respir. Crit. Care Med., May 15, 2007; 175(10): 975 - 976.
[Full Text] [PDF]

M. Oostendorp, U. F.H. Engelke, M. A.A.P. Willemsen, and R. A. Wevers
Diagnosing Inborn Errors of Lipid Metabolism with Proton Nuclear Magnetic Resonance Spectroscopy
Clin. Chem., July 1, 2006; 52(7): 1395 - 1405.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

All Versions of this Article:
clinchem.2003.020214v1
50/1/58 most recent

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 (22)

Citing Articles via Google Scholar

Google Scholar

Articles by Engelke, U. F.H.

Articles by Wevers, R. A.

Search for Related Content

PubMed

PubMed Citation

Articles by Engelke, U. F.H.

Articles by Wevers, R. A.

Related Collections

Molecular Diagnostics and Genetics

				N. Shanaiah, M. A. Desilva, G. A. Nagana Gowda, M. A. Raftery, B. E. Hainline, and D. Raftery Class selection of amino acid metabolites in body fluids using chemical derivatization and their enhanced 13C NMR PNAS, July 10, 2007; 104(28): 11540 - 11544. [Abstract] [Full Text] [PDF]

				J. Hunt If It Smells Like a Duck, It Might Be an Asthma Subphenotype Am. J. Respir. Crit. Care Med., May 15, 2007; 175(10): 975 - 976. [Full Text] [PDF]

				M. Oostendorp, U. F.H. Engelke, M. A.A.P. Willemsen, and R. A. Wevers Diagnosing Inborn Errors of Lipid Metabolism with Proton Nuclear Magnetic Resonance Spectroscopy Clin. Chem., July 1, 2006; 52(7): 1395 - 1405. [Abstract] [Full Text] [PDF]