Presence of Protein Fragments in Urine of Critically Ill Patients with Acute Renal Failure: A Nephrologic Enigma

Giusti, Massimo; Cantaluppi, Vincenzo; Fenocchio, Chiara; Motta, Daria; Masini, Sergio; Pacitti, A; Lanfranco, Giacomo

doi:10.1373/clinchem.2004.037077

Cited by 4 publications

(2 citation statements)

References 18 publications

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“…From quantitative LC-MS/MS analysis, we have been able to detect AGE (and oxidation adduct) enrichment on low molecular mass peptides in vivo only in portal venous plasma of human subjects and not in peripheral venous plasma (18,33). Peptides from incomplete proteolysis are found in vivo (34,35) but our LC-MS/MS analysis indicates that, except in portal venous plasma, they are not enriched with glycation, oxidation, or nitration adduct residues. Some glycation free adducts have been detected previously: for example, plasma pentosidine in uremia as an indicator of dialysis efficiency (36).…”

Section: Quantitation Of Glycation Adducts In Uremia — the Advantages Of Liquid Chromatography With Tandem Mass Spectrometric (Lc-ms/ms) mentioning

confidence: 73%

Measurement of Protein Glycation, Glycated Peptides, and Glycation Free Adducts

Thornalley

2005

Perit Dial Int

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Protein glycation adducts, early glycation adducts, such as N∊-fructosyl-lysine, and advanced glycation end products (AGEs) are uremic toxins. Glycation adducts are found in plasma and tissue proteins (glycation adduct residues), in peptides (glycation adduct peptide residues), and glycated amino acids (glycation free adducts). The latter two analyte groups arise from proteolysis of glycated proteins and glycation of peptides and amino acids. Quantitation of glycation adducts in uremia is difficult because of the presence of many different AGEs at low concentrations in different forms in the presence of many potential interferences. Application of liquid chromatography with tandem mass spectrometric (LC-MS/MS) detection to plasma, urine, and dialysate samples of uremic patients has provided a comprehensive and quantitative analysis of glycation adducts in uremia. Glycation free adducts accumulate markedly in the plasma of uremic patients and are eliminated in the peritoneal dialysate. Multiple glycation adducts, and also protein oxidation and nitration adducts, may be quantified concurrently. Glycation free adducts are the major form of glycation adduct eliminated in dialysate. LC-MS/MS may now be used to quantify concentrations, extents of protein modification, clearances, and excretion rates of glycation adducts in uremia.

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Section: Quantitation Of Glycation Adducts In Uremia — the Advantages Of Liquid Chromatography With Tandem Mass Spectrometric (Lc-ms/ms) mentioning

confidence: 73%

Measurement of Protein Glycation, Glycated Peptides, and Glycation Free Adducts

Thornalley

2005

Perit Dial Int

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“…It can produce many distinct low molecular mass species from a particular higher molecular mass protein. The fragmentation pattern may reflect different pathogenic processes, and protein fragments have already been recognized as diagnostic and prognostic biomarkers in different types of cancer, renal and connective tissue diseases, etc (34, 39, 40). Bearing in mind many limitations of this study regarding selection of fPSA-immunoreactive fragments as well as sample heterogeneity in distinct groups, the results obtained add new value to low molecular mass PSA-immunoreactive species in sera.…”

Section: Discussionmentioning

confidence: 99%

Human Serum Low Molecular Mass Prostate-Specific Antigen as Biomarker

Goč

Janković

2017

Journal of Medical Biochemistry

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SummaryBackground: Prostate-specific antigen (PSA) is a glycoprotein tumor marker known to exist as numerous glycospecies. Investigations on its glycobiochemical properties aimed at their use in the preparation of adjuncts in determining PSA concentration for clinical purposes have accumulated a lot of data on its structural properties. In this study, we reconsidered unexplored ubiquitously present low molecular mass species of PSA regarding to molecular mass, origin and pathophysiological source specificity in order to evaluate them as biomarkers. Methods: Data on low molecular mass PSA-immunoreactive species from sera of subjects with prostate cancer (PCa), benign prostatic hyperplasia (BPH), breast cancer (BCa), and urine of healthy males obtained by on-chip immunoaffinity chromatography combined with mass spectrometry were analyzed. Results: The results obtained indicated PSA species common to BCa, PCa, and BPH at 12-13 kDa, 17-19 kDa and 21-24 kDa. The striking difference in predominant frequencies made the profile characteristic in each examined pathophysiological condition. On the other hand, paired groups of prostatic and extraprostatic PSA contained rare species with small differences among groups concerning individual species. Low molecular mass PSA also included rare species unique for each group of samples. Conclusions: The results obtained revealed that uniformity of low molecular mass PSA-immunoreactive species in sera prevails over diversity related to cancer and non-cancer conditions, but at the same time some of them are molecules with biomarker potential for BPH detection.

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The significance of tubular and glomerular proteinuria in critically ill patients with severe acute kidney injury

Lim¹,

Tan²,

Lau³

1969

Pak J Med Sci

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Objective: Critically ill patients with acute kidney injury (AKI) frequently need acute renal replacement therapy (aRRT). We evaluated an inexpensive, rapid quantitative and qualitative analysis of proteinuria on the course of AKI patients requiring aRRT in intensive care. Method: This was a prospective, observational study of critically ill patients with severe established AKI or Acute on Chronic Kidney Injury (AoCKI) requiring aRRT. Urine samples were analyzed using Sodium-Dodecyl-Sulphate-Polyacryamide Gel Electrophoresis (SDS-PAGE). Results: A total of 30 critically ill patients were studied. Those who died have higher APACHE II (29 ± 6 vs. 20 ± 5, p<0.001), multi-organ failure (0.7 ± 0.5 vs. 0.2 ± 0.4, p < 0.02) and Tubular/Glomerular ratio (114 ± 60 vs. 75± 37, p < 0.05).The renal non-recoverers have higher baseline creatinine (415 ± 328 vs. 125± 19 umol/l, p < 0.01), urinary Dipstick value (1.8±0.8 vs. 0.5±0, p <0.05) and Glomerular score (3.0 ± 1.8 vs. 0.6 ± 0.2, p < 0.02).Heavy tubular proteinuria also predicts a longer duration of interim dialysis support and mortality whereas glomerular proteinuria correlates with development of chronicity and End Stage Renal Disease (ESRD). Conclusions: The dominant presence of tubular proteinuria is associated with poor survival in patients who have high APACHE II score and multi-organ failure. It also correlates with a longer duration of dialysis support in survivals. Renal Non-recoverers had heavy dominant presence of glomerular proteinuria. SDS-PAGE proteinuria analysis offers a reliable and inexpensive method to prognosticate proteinuria in this group of critically ill patients.

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Presence of Protein Fragments in Urine of Critically Ill Patients with Acute Renal Failure: A Nephrologic Enigma

Cited by 4 publications

References 18 publications

Measurement of Protein Glycation, Glycated Peptides, and Glycation Free Adducts

Measurement of Protein Glycation, Glycated Peptides, and Glycation Free Adducts

Human Serum Low Molecular Mass Prostate-Specific Antigen as Biomarker

The significance of tubular and glomerular proteinuria in critically ill patients with severe acute kidney injury

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