Monoclonal immunoglobulins, also known as paraproteins,

Transcription

1 Paraproteins Are a Common Cause of Interferences With Automated Chemistry Methods Yusong Yang, MD, PhD; Peter J. Howanitz, MD; Joan H. Howanitz, MD; Helen Gorfajn, MS; Keung Wong, MS Context. Previous studies have shown that paraproteins caused spurious results on individual analytes including total bilirubin (TBIL), direct bilirubin (DBIL), or HDL-cholesterol (HDL-C). Studies demonstrating paraprotein interferences with multiple analytes measured by different analyzers have not been reported. Objective. To systemically investigate interferences of paraproteins on TBIL, DBIL, and HDL-C measured by the Roche MODULAR and the Olympus AU2700. Design. Eighty-eight serum specimens with monoclonal gammopathies were analyzed using the Roche MOD- ULAR and the Olympus AU2700. Paraprotein interferences with the MODULAR and AU2700 were identified by abnormal absorbance curves and confirmed by results from the Ortho Vitros 950 or inconsistent laboratory information. Results. Spurious results occurred in 89 of 528 measurements; 29 specimens did not demonstrate any interferences whereas 26 specimens gave spurious results in 2 to 4 of the 6 assays. Paraprotein interferences caused spuriously high levels of TBIL in 4 sera measured by the MOD- ULAR. In contrast, paraprotein interferences on DBIL were observed by at least 1 method in 44% (39/88) of sera assayed, occurring almost exclusively with the AU2700. Paraprotein interferences with HDL-C results were present in 35% of specimens assayed with the MODULAR and 16% of specimens assayed with the AU2700. In specimens with interferences, spuriously low AU2700 DBIL, MODULAR HDL-C, and AU2700 HDL-C results occurred with 28%, 90%, and 91% of specimens, respectively. Conclusions. We demonstrated that paraprotein interferences with TBIL, DBIL, and HDL-C are relatively common and provided explanations why these interferences occurred. Although it is difficult to predict which specimens cause interferences, spurious results appeared method and concentration dependent. (Arch Pathol Lab Med. 2008;132: ) Monoclonal immunoglobulins, also known as paraproteins, have been reported to interfere with a number of routine chemistry methods including analyses for creatinine, 1,2 C-reactive protein, 3 glucose, 4 iron, 5,6 inorganic phosphate, 7 9 and uric acid. 10 Recent studies have shown that paraproteins caused false-positive results for total bilirubin (TBIL) and direct bilirubin (DBIL) 14 and falsenegative results for HDL-cholesterol (HDL-C). 12,15 19 The frequency of paraprotein interferences with these analytes on automated chemistry analyzers was reported to be very rare, and comparative studies of paraprotein interferences with TBIL, DBIL, and HDL-C have not been reported with major automated chemistry analyzers. These interferences may cause incorrect diagnoses, inappropriate treatments, longer hospital stays, and increased morbidity in patients who already may be gravely ill. We systemically investigated the potential interference of paraproteins on measurements of TBIL, DBIL, and HDL-C using Accepted for publication October 12, From the Department of Pathology, State University of New York Downstate Medical Center, Brooklyn, NY (Drs Yang, P. J. Howanitz, and J. H. Howanitz, and Ms Gorfajn); and Institute of Pathology, Clinical Chemistry Laboratory, Kings County Hospital Center, Brooklyn, NY (Mr Wong). The authors have no relevant financial interest in the products or companies described in this article. Reprints: Yusong Yang, MD, PhD, Department of Pathology, Box 24, State University of New York Downstate Medical Center, 450 Clarkson Ave, Brooklyn, NY ( yusong.yang@downstate.edu). 88 serum specimens collected from patients with monoclonal gammopathies and measured using 2 commonly used automated chemistry analyzers. MATERIALS AND METHODS This study was conducted as part of a laboratory performance improvement program for patient result reporting. Serum specimens were collected from patients with monoclonal gammopathies determined by serum protein electrophoretic and immunofixation studies during a 1-year period. The sera were free of hemolysis, icterus, and lipemia by routine index checks on automated analyzers. None of the specimens were duplicates or triplicates; if they were from the same patients, they were obtained at different times. Serum protein electrophoretic and immunofixation studies were performed using the SPIFE 3000 (Helena Laboratories, Beaumont, Tex), and serum total protein concentrations were determined with the Roche P800 MODULAR (Roche Diagnostics, Indianapolis, Ind). Paraprotein concentrations were quantitated by the Quickscan 2000 (Helena Laboratories). Serum levels of TBIL, DBIL, and HDL-C were measured independently using the Roche P800 MODULAR, Olympus AU2700 (Olympus Diagnostics, Melville, NY), and Vitros 950 (Ortho-Clinical Diagnostics, Rochester, NY) automated chemistry analyzers. Paraprotein interferences with the Roche MODULAR and Olympus AU2700 were identified by an abnormal reaction absorbance curve obtained directly from the reaction monitor integrated into the automated analyzers and confirmed by at least 1 additional finding. Absorbance curve data from the Olympus AU2700 printouts were plotted manually, whereas similar data Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al 217

2 Figure 1. Scatter plot of total bilirubin (TBIL) concentrations measured by 2 automated chemistry analyzers., Specimens without interferences by paraproteins;, specimens displaying interferences by paraproteins measured by the Roche MODULAR. * To convert to SI units in micromoles per liter, multiply values in milligrams per deciliter by from the Roche MODULAR were used directly. Because it had been shown that the Vitros 950 did not provide spurious results for DBIL and TBIL, it was used for confirmation of interferences. 12,14,16 The Ektachem slide method used in the Vitros 950 was interference free because the specimens had to penetrate through several layers before reaching the reaction layer, and the interfering compounds were probably filtered out. 20 Therefore, when potential interferences were identified and an adequate specimen remained, confirmation of the spurious results was made by additional measurements using the Vitros 950, except for HDL-C, as our instrument did not have this method included in its test menu. Paraprotein interferences also were confirmed by specimens with negative DBIL or negative HDL-C results, specimens with abnormally high TBIL levels from nonicteric patients without evidence of liver diseases and hemolysis, or specimens with DBIL levels higher than TBIL levels. The Roche MODULAR TBIL assay is a chromogenic 2-point end point assay modified from the diazo method 21 that is performed in 1 cuvette. First the patient s serum is incubated with reagent 1 (R1), which contains surfactant to accelerate the reaction and to solubilize protein. Then, reagent 2 (R2) containing a diazonium salt and HCl is added to produce azobilirubin, which is red under acidic conditions. Before R1 is added, the serum specimen should not be turbid. In contrast, the Olympus AU2700 TBIL assay is a 2-cuvette, 1-point end point assay that uses similar reagents. Both the reaction cuvette and the blank cuvette contain surfactant, whereas the chromogen is not added to the blank cuvette. The Roche MODULAR and Olympus AU2700 DBIL assays resemble their manufacturers TBIL assays, other than that a solubilizing agent such as surfactant is not added. When paraprotein interferences with DBIL initially were suspected in the specimens with either negative DBIL values or DBIL concentrations higher than TBIL concentrations, they subsequently were confirmed by abnormal reaction absorbance curves. The Roche HDL-C Plus second-generation assay and the Olympus HDL-C assay are 2-reagent homogenous systems for the selective measurement of serum HDL-C in the presence of other lipoprotein particles. Reagent 1 (R1) selectively forms colorless water-soluble complexes with non-hdl lipoprotein, which is protected from subsequent enzymatic reactions. The HDL-C is then determined enzymatically by the addition of R2 containing cholesterol esterase, cholesterol oxidase, and a chromogen system into the reaction mixture. The HDL-C concentration is determined by the absorbance after the addition of R2 subtracted from the baseline absorbance in the presence of R1. RESULTS The present study included 88 serum specimens from 52 patients with monoclonal gammopathies treated at a major municipal hospital or a university hospital. The paraprotein concentrations of these specimens ranged from 0.5 to 8.9 g/dl with a mean of 3.67 g/dl. The majority (60%) of the paraproteins were immunoglobulin (Ig) G, 18% were IgG, 11% were IgA, and 7% were IgM. Specimens with paraprotein concentrations less than 3.0 g/dl had spurious results in 7.2% of assays; when paraprotein concentrations were 3.0 to 5.0 g/dl, spurious results were seen in 22.4% of assays, and when paraprotein concentrations were greater than 5.0 g/dl, spurious results were seen in 31.3% of assays. Spurious results occurred in 89 of 528 measurements; 29 specimens did not demonstrate any interferences, whereas 26 specimens gave spurious results in 2 to 4 of the 6 assays. Of 88 serum specimens, 4 specimens (4.3%) from 3 patients with monoclonal gammopathies displayed spuriously high Roche MODULAR TBIL concentrations. The interferences in 3 specimens initially were suggested by nonicteric sera with abnormally high TBIL values of greater than 25 mg/dl (428 mol/l), (Figure 1) and subsequently were identified and confirmed along with a fourth specimen by abnormal reaction absorbance curves (Figure 2, C and D) compared with those obtained from normal control serum (Figure 2, A), measurements by the Vitros 950, and icteric serum without measurable paraproteins (Figure 2, B). In our study, the interferences were found exclusively in specimens from patients with IgG or IgG monoclonal gammopathies, and in these 4 specimens, the paraprotein concentrations (mean, 5.45 g/dl) were higher than the overall mean of the 88 monoclonal proteins studied. When we manually performed the Roche MODULAR TBIL assay in test tubes according to manufacturer s suggested protocol using a specimen with the suspected in- 218 Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al

3 Figure 2. Reaction absorbance curves of the Roche MODULAR total bilirubin (TBIL) assay monitored. A, Normal control serum. B, An icteric patient serum without paraprotein. C and D, Nonicteric, nonhemolytic serum specimens containing paraproteins. The gray vertical bars indicate the points at which measurements are taken to calculate results. IgG indicates immunoglobulin G. terference, the specimen was slightly turbid visually before adding R1 but became clear after the addition of R1. However, the addition of R2 caused the reaction mixture to become clear instead of the red translucent appearance observed with the control patient s specimens. When the TBIL concentrations of these sera were measured independently by the Olympus AU2700 and Vitros 950 automated chemistry analyzers, no interferences were identified with these 2 instruments. Using the criteria we established for interference, 39 (44%) of 88 specimens were found to display interferences with DBIL on the Olympus AU2700 (Figure 3). However, only 1 specimen was found to have interferences with DBIL when measured by the Roche MODULAR, and this result was confirmed as spurious by the Vitros 950. We found that these interferences occurred when the reaction absorbance curve of the blank cuvette (DBIL-B) did not parallel the absorbance curve of the reaction cuvette (DBIL-C) (Figure 4). The Olympus instrument was programmed to subtract the absorbance of the blank cuvette from the absorbance of the reaction cuvette at the end point, then tally the difference and convert this difference into a numerical result. If the absorbance of the blank cuvette was lower than the end point absorbance of the reaction cuvette, the instrument reported a positive value (Figure 4, A); in contrast, if the absorbance of the Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al 219

4 Figure 3. Scatter plot of direct bilirubin (DBIL) measurements made by 2 automated chemistry analyzers., Specimens without evidence of paraprotein interferences;, specimens displaying interferences by paraproteins measured by the Olympus AU2700;, specimens displaying interferences by paraproteins measured by the Olympus AU2700 and the Roche MODULAR. * For SI units in micromoles per liter, multiply results in milligrams per deciliter by blank cuvette was higher than the end point absorbance of the reaction cuvette, the instrument reported a negative value (Figure 4, B). Among the 39 specimens with Olympus AU2700 DBIL interferences, 14 specimens had spuriously high values and 25 specimens had spuriously low values. However, the specimens displaying interferences with the Olympus AU2700 DBIL method tended to give irreproducible DBIL values, as demonstrated by a specimen that varied from falsely positive (13.0 mg/dl [222 mol/l]) to falsely negative ( 17.3 mg/dl [296 mol/l]) values when measured repeatedly (data not shown). Figure 5 depicts 31 (35%) of 88 specimens that demonstrated HDL-C interferences with the Roche MODULAR, and of these, 90% were spuriously low. In contrast, 14 (16%) of 88 specimens demonstrated HDL-C interferences when measured by the Olympus AU2700. Of these interfering sera, 7 demonstrated interferences with both methods. Examples of absorbance curves demonstrating interferences with HDL-C as identified by abnormal reaction absorbance curves compared with those from control specimens and confirmed by negative HDL-C values are shown in Figure 6. In Figure 6, B and C, the Roche MOD- ULAR absorbance values of the blank obtained just before the addition of R2 were higher than after the addition of R2, thereby giving spurious results. There was a much higher baseline absorbance before the addition of R2 in the specimens displaying interferences with the Olympus AU2700 HDL-C method compared Figure 4. Absorbance curves from the Olympus AU2700 direct bilirubin (DBIL) assay. A and B, Abnormal reaction absorbance curves of the Olympus AU2700 DBIL assay from 2 patient specimens containing paraproteins. The DBIL assay is a 2-cuvette, end point assay utilizing a sample blank; the sample blank cuvette (DBIL-B) absorbance is subtracted from the color cuvette (DBIL-C) absorbance to determine the net reaction absorbance. The arrows indicate reaction end point. 220 Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al

5 Figure 5. Scatter plot of high-density lipoprotein cholesterol (HDL-C) measurements made by 2 automated chemistry analyzers., Specimens without evidence of paraprotein interferences;, specimens displaying interferences by paraproteins measured by the Roche MODULAR;, specimens displaying interferences by paraproteins measured by the Olympus AU2700; #, specimens displaying interferences by paraproteins measured by the Roche MODULAR and the Olympus AU2700. * For SI units in millimoles per liter, multiply results in milligrams per deciliter by with that in the control specimens; after the addition of R2, absorbance values did not increase as much as expected (Figure 6, D), thereby accounting for the spuriously low values of HDL-C. Visually checking cuvettes containing specimens with the interference also demonstrated white precipitates that were formed after the addition of R1. The paraprotein interferences appear to be concentration dependent, as dilution of patient sera and treatment of the patient by therapeutic plasmapheresis or chemotherapeutic agents causing decreasing monoclonal proteins minimized paraprotein interferences (data not shown). COMMENT Our studies demonstrate that the interferences with TBIL, DBIL, and HDL-C are relatively common in the presence of paraproteins. Comparing results among different analyzers and monitoring absorbance curves led us to conclude that paraprotein interferences are more prevalent than previously reported. Pantanowitz and coworkers 11 found that artifactual TBIL occurred in 2 (1.2%) of 115 patient sera, whereas Nauti et al 14 reported that paraprotein interferences with the Olympus AU2700 DBIL were observed in only 3 (1.5%) of 200 serum specimens. Spuriously low levels of HDL-C on the Roche 917 analyzer caused by paraprotein were found in 2 (13%) of 15 specimens at a major medical center. 12 To our knowledge, paraprotein interferences with HDL-C measured by the Olympus automated chemistry analyzers have not been reported. Our study revealed that the incidence of paraprotein interference with the Olympus AU2700 and Roche MOD- ULAR DBIL assays was 16% and 35%, respectively, in 88 serum specimens. We also found that paraproteins interfere with Olympus AU2700 HDL-C, although the frequency (16%) was not as high as that on the Roche MODULAR (35%). Specimens that gave spurious results in one assay had a high likelihood of yielding a spurious result in other assays. A recent study showed that paraprotein caused only spuriously high levels with Olympus AU2700 DBIL measurements. 14 However, in contrast, our study demonstrated that most DBIL interferences (64%) were spuriously low when measured by the Olympus AU2700 DBIL. Because the Olympus DBIL assay gave exceedingly variable repetitive results ranging from a markedly positive to markedly negative interferences in specimens containing a monoclonal protein, we believe that describing an interference as negative or positive is unsatisfactory. The paraprotein interferences with TBIL, DBIL, and HDL-C appeared to be method dependent. The interferences with TBIL and HDL-C mainly were observed with the Roche MODULAR, while DBIL interferences occurred most frequently with the Olympus AU2700. The Roche TBIL assay is a 1-cuvette, 2-point end point assay. Because the addition of R2 to the reaction mixture changed the assay conditions to more acidic (ph 1 2), paraproteins could form insoluble complexes with R2, which cause the interferences. On the other hand, the Olympus TBIL assay is a 2-cuvette end point assay. Both cuvettes, the sample blank cuvette and the reaction cuvette, contain the same reagents, except the chromogen is only in the reaction cuvette. Therefore, the condition in the assay is not changed as there is no addition of R2. The chromogenic reaction of the DBIL assay occurs at a verylowph( 1). A protein stabilizing agent is included to avoid protein precipitation. It appears that the solubilization capacity of the Olympus AU2700 protein stabilizing agent is not sufficient to prevent the proteins in solution from precipitating at such an acidic ph, which may cause more interferences with DBIL on the Olympus AU2700. As mentioned in the Results, spuriously low HDL-C results observed in the patients with monoclonal gammopathies on the Roche MODULAR and the Olympus AU2700 may be due to the high baseline absorbance in the presence of R1 reagent. The R1 reagent contains a buffer system to selectively form a water-soluble complex Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al 221

6 Figure 6. Comparison of high-density lipoprotein cholesterol (HDL-C) measurements made by 2 automated chemistry analyzers; the Roche MODULAR (A through C) and the Olympus AU2700 (D) HDL-C assay absorbance curves. A, A control patient serum. B and C, Serum specimens containing paraproteins. The gray vertical bars indicate the points at which measurements were taken to calculate results. D, Reaction absorbance curve of the Olympus AU2700 HDL-C assay. The arrows indicate photometric points at which R1 (point 0) and R2 (point 10) reagents were added. The reaction stops at photometric point 27. IgG indicates immunoglobulin G. with low-density lipoprotein, very low-density lipoprotein, and chylomicrons. It may be that the differences of the components or concentrations of the components of the buffer system in the Roche MODULAR and Olympus AU2700 HDL-C assays caused more interferences with HDL-C to be observed on the Roche MODULAR. Our studies demonstrate that paraprotein interferences with DBIL and HDL-C are relatively common, and spurious results of TBIL, DBIL, and HDL-C appear to be methodology and concentration dependent. In a few patients followed for a period of time, treatment that decreased paraprotein concentrations caused interferences to disappear, while disease progression and increasing monoclonal protein concentrations caused interferences to increase. It is important to appreciate the occurrence of these interferences to avoid misinterpretation of the results, especially because low HDL-C ( 40 mg/dl [684 mol/l]) is considered to be an independent risk factor for coronary heart disease. 22 To automatically detect the interference, Smogorzewska et al 12 suggested manually programming the analyzer to trigger a flag when the difference of absorbance between certain points was above a 222 Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al

7 preset value for the Roche MODULAR TBIL assay or the absorbance immediately before the addition of the R2 agent was above a designated value for the Roche AU2700 HDL-C assay. This may help when the abnormal absorbance reaction curves follow a similar kinetic pattern. However, our studies showed that the abnormal reaction curves of the Roche MODULAR TBIL assay and the Olympus AU2700 DBIL assay have different patterns (Figures 2 and 4), which may lead to missing some interferences if a programmable rule is used. An approach that we favor for bilirubin assays is to program the analyzer to automatically flag results for confirmation when specimens have TBIL results greater than 20 mg/dl (342 mol/l) and the icteric flag is not markedly positive. 13 To prevent results preceded by a negative sign from being reported, we recommend programming the laboratory information system to reject patient DBIL and HDL-C results that are preceded by a minus sign. In conclusion, we found that paraprotein interferences with clinical laboratory measurements are far more frequent than previously reported. If an interference occurs with one assay, it is likely that other assays also will be affected. These types of interferences appear in part to be concentration dependent. Specimens with paraproteins cause spurious results by causing precipitation in TBIL, DBIL, and HDL-C assays. References 1. Datta P, Graham GA, Schoen I. Interference by IgG paraproteins in the Jaffe method for creatinine determination. Am J Clin Pathol. 1986;85: Hummel KM, von Ahsen N, Kuhn RB, et al. Pseudohypercreatininemia due to positive interference in enzymatic creatinine measurements caused by monoclonal IgM in patients with Waldenstrom s macroglobulinemia. Nephron. 2000; 86: Yu A, Pira U. False increase in serum C-reactive protein caused by monoclonal IgM-lambda: a case report. Clin Chem Lab Med. 2001;39: Dimeski G, Carter A. Rare IgM interference with Roche/Hitachi modular glucose and gamma-glutamyltransferase methods in heparin samples. Clin Chem. 2005;51: Dorizzi R, Battaglia P, Lora A. Iron measurement in patients with monoclonal immunoglobulin: a further caution. Clin Chem. 1991;37: Bakker AJ. Influence of monoclonal immunoglobulins in direct determinations of iron in serum. Clin Chem. 1991;37: Sinclair D, Smith H, Woodhead P. Spurious hyperphosphataemia caused by an IgA paraprotein: a topic revisited. Ann Clin Biochem. 2004;41: Barutcuoglu B, Parildar Z, Mutaf I, Habif S, Bayindir O. Spuriously elevated inorganic phosphate level in a multiple myeloma patient. Clin Lab Haematol. 2003;25: Savory DJ, Pearce CJ. Paraprotein interference causing pseudohyperphosphataemia: evaluation of an improved methodology. Ann Clin Biochem. 1995; 32: Langman LJ, Allen LC, Romaschin AD. Interference of IgM paraproteins in the Olympus AU800 uric acid assay. Clin Biochem. 1998;31: Pantanowitz L, Horowitz GL, Upalakalin JN, Beckwith BA. Artifactual hyperbilirubinemia due to paraprotein interference. Arch Pathol Lab Med. 2003; 127: Smogorzewska A, Flood JG, Long WH, Dighe AS. Paraprotein interference in automated chemistry analyzers. Clin Chem. 2004;50: Sheppard CA, Allen RC, Austin GE, et al. Paraprotein interference in automated chemistry analyzers. Clin Chem. 2005;51: Nauti A, Barassi A, Merlini G, d Eril GV. Paraprotein interference in an assay of conjugated bilirubin. Clin Chem. 2005;51: Bakker AJ, Zijlstra A, Leemhuis MP. False negative results in the Roche assay for HDL-cholesterol. Ann Clin Biochem. 2003;40: Kadri N, Douville P, Lachance P. Monoclonal paraprotein may interfere with the Roche Direct HDL-C Plus assay. Clin Chem. 2002;48: Tsai LY, Tsai SM, Lee SC, Liu SF. Falsely low LDL-cholesterol concentrations and artifactual undetectable HDL-cholesterol measured by direct methods in a patient with monoclonal paraprotein. Clin Chim Acta. 2005;358: Berth M, Delangehe J. Protein precipitation as a possible important pitfall in the clinical chemistry analysis of blood samples containing monoclonal immunoglobins: 2 case reports and a review of the literature. Acta Clin Belg. 2004; 59: Baca A, Haber RJ, Susishi K, Frost PH, Ng VN. Artifactual undetectable HDL-cholesterol with the Beckman Synchron LX and Vitros 950 assays temporally associated with a paraprotein. Clin Chem. 2004;50: Zaman Z, Sneyers L, Van Orshoven A, Blanckaert N, Marien G. Elimination of paraprotein interference in determination of plasma inorganic phosphate by ammonium molybdate method. Clin Chem. 1995;41: Westwood A. The analysis of bilirubin in serum. Ann Clin Biochem. 1991; 28: Expert Panel on Detection, Evaluation, and Treatment of High Blood Cholesterol in Adults. Executive Summary of The Third Report of The National Cholesterol Education Program (NCEP) Expert Panel on Detection, Evaluation, and Treatment of High Blood Cholesterol in Adults (Adult Treatment Panel III). JAMA. 2001;285: Arch Pathol Lab Med Vol 132, February 2008 Paraprotein Interferences With Automated Methods Yang et al 223