Effects of sample dilution, peroxidase concentration, and chloride ion on the measurement of unbound bilirubin in premature newborns
To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl −) on plasma unbound bilirubin ( B f) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns. B f was measured with a UB Analyzer in 74 samples...
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Published in | Clinical biochemistry Vol. 40; no. 3; pp. 261 - 267 |
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Main Authors | , , , , , , |
Format | Journal Article |
Language | English |
Published |
United States
Elsevier Inc
01.02.2007
|
Subjects | |
Online Access | Get full text |
ISSN | 0009-9120 1873-2933 |
DOI | 10.1016/j.clinbiochem.2006.09.006 |
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Abstract | To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl
−) on plasma unbound bilirubin (
B
f) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns.
B
f was measured with a UB Analyzer in 74 samples at the standard 42-fold sample dilution and compared with
B
f measured at a 2-fold sample dilution using a FloPro Analyzer.
B
f was measured at two peroxidase concentrations to determine whether the peroxidase steady state
B
f (
B
fss) measurements were significantly less than the equilibrium
B
f (
B
feq), in which case it was necessary to calculate
B
feq from the two
B
fss measurements.
B
f was also measured before and after adding 100 mmol/L Cl
− to the UB Analyzer assay buffer.
B
feq at the 42-fold dilution was nearly 10-fold less than but it correlated significantly with
B
feq at the 2-fold dilution (mean 8.2
±
5.2 nmol/L versus 73.5
±
70 nmol/L, respectively,
p
<
0.0001; correlation
r
=
0.6). The two UB Analyzer
B
fss measurements were significantly less than
B
feq in 42 of 74 (57%) samples, and Cl
− increased
B
feq in 66 of 74 (89%) samples by a mean of 82
±
67%.
B
fss measured by the UB Analyzer at the standard 42-fold sample dilution using assay buffer without Cl
− and a single peroxidase concentration is significantly less than the
B
feq in undiluted plasma. Accurate
B
f measurements can be made only in minimally diluted serum or plasma. |
---|---|
AbstractList | To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl(-)) on plasma unbound bilirubin (B(f)) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns.OBJECTIVESTo assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl(-)) on plasma unbound bilirubin (B(f)) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns.B(f) was measured with a UB Analyzer in 74 samples at the standard 42-fold sample dilution and compared with B(f) measured at a 2-fold sample dilution using a FloPro Analyzer. B(f) was measured at two peroxidase concentrations to determine whether the peroxidase steady state B(f) (B(fss)) measurements were significantly less than the equilibrium B(f) (B(feq)), in which case it was necessary to calculate B(feq) from the two B(fss) measurements. B(f) was also measured before and after adding 100 mmol/L Cl(-) to the UB Analyzer assay buffer.DESIGN AND METHODSB(f) was measured with a UB Analyzer in 74 samples at the standard 42-fold sample dilution and compared with B(f) measured at a 2-fold sample dilution using a FloPro Analyzer. B(f) was measured at two peroxidase concentrations to determine whether the peroxidase steady state B(f) (B(fss)) measurements were significantly less than the equilibrium B(f) (B(feq)), in which case it was necessary to calculate B(feq) from the two B(fss) measurements. B(f) was also measured before and after adding 100 mmol/L Cl(-) to the UB Analyzer assay buffer.B(feq) at the 42-fold dilution was nearly 10-fold less than but it correlated significantly with B(feq) at the 2-fold dilution (mean 8.2+/-5.2 nmol/L versus 73.5+/-70 nmol/L, respectively, p<0.0001; correlation r=0.6). The two UB Analyzer B(fss) measurements were significantly less than B(feq) in 42 of 74 (57%) samples, and Cl(-) increased B(feq) in 66 of 74 (89%) samples by a mean of 82+/-67%.RESULTSB(feq) at the 42-fold dilution was nearly 10-fold less than but it correlated significantly with B(feq) at the 2-fold dilution (mean 8.2+/-5.2 nmol/L versus 73.5+/-70 nmol/L, respectively, p<0.0001; correlation r=0.6). The two UB Analyzer B(fss) measurements were significantly less than B(feq) in 42 of 74 (57%) samples, and Cl(-) increased B(feq) in 66 of 74 (89%) samples by a mean of 82+/-67%.B(fss) measured by the UB Analyzer at the standard 42-fold sample dilution using assay buffer without Cl(-) and a single peroxidase concentration is significantly less than the B(feq) in undiluted plasma. Accurate B(f) measurements can be made only in minimally diluted serum or plasma.CONCLUSIONSB(fss) measured by the UB Analyzer at the standard 42-fold sample dilution using assay buffer without Cl(-) and a single peroxidase concentration is significantly less than the B(feq) in undiluted plasma. Accurate B(f) measurements can be made only in minimally diluted serum or plasma. To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl −) on plasma unbound bilirubin ( B f) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns. B f was measured with a UB Analyzer in 74 samples at the standard 42-fold sample dilution and compared with B f measured at a 2-fold sample dilution using a FloPro Analyzer. B f was measured at two peroxidase concentrations to determine whether the peroxidase steady state B f ( B fss) measurements were significantly less than the equilibrium B f ( B feq), in which case it was necessary to calculate B feq from the two B fss measurements. B f was also measured before and after adding 100 mmol/L Cl − to the UB Analyzer assay buffer. B feq at the 42-fold dilution was nearly 10-fold less than but it correlated significantly with B feq at the 2-fold dilution (mean 8.2 ± 5.2 nmol/L versus 73.5 ± 70 nmol/L, respectively, p < 0.0001; correlation r = 0.6). The two UB Analyzer B fss measurements were significantly less than B feq in 42 of 74 (57%) samples, and Cl − increased B feq in 66 of 74 (89%) samples by a mean of 82 ± 67%. B fss measured by the UB Analyzer at the standard 42-fold sample dilution using assay buffer without Cl − and a single peroxidase concentration is significantly less than the B feq in undiluted plasma. Accurate B f measurements can be made only in minimally diluted serum or plasma. To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl(-)) on plasma unbound bilirubin (B(f)) measurements made using a commercial peroxidase methodology (UB Analyzer) in a study population of ill, premature newborns. B(f) was measured with a UB Analyzer in 74 samples at the standard 42-fold sample dilution and compared with B(f) measured at a 2-fold sample dilution using a FloPro Analyzer. B(f) was measured at two peroxidase concentrations to determine whether the peroxidase steady state B(f) (B(fss)) measurements were significantly less than the equilibrium B(f) (B(feq)), in which case it was necessary to calculate B(feq) from the two B(fss) measurements. B(f) was also measured before and after adding 100 mmol/L Cl(-) to the UB Analyzer assay buffer. B(feq) at the 42-fold dilution was nearly 10-fold less than but it correlated significantly with B(feq) at the 2-fold dilution (mean 8.2+/-5.2 nmol/L versus 73.5+/-70 nmol/L, respectively, p<0.0001; correlation r=0.6). The two UB Analyzer B(fss) measurements were significantly less than B(feq) in 42 of 74 (57%) samples, and Cl(-) increased B(feq) in 66 of 74 (89%) samples by a mean of 82+/-67%. B(fss) measured by the UB Analyzer at the standard 42-fold sample dilution using assay buffer without Cl(-) and a single peroxidase concentration is significantly less than the B(feq) in undiluted plasma. Accurate B(f) measurements can be made only in minimally diluted serum or plasma. |
Author | Stevenson, David K. Ahlfors, Charles E. Vreman, Hendrik J. Wong, Ronald J. Oh, William Bender, G. Jesse Morris, Brenda H. |
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BackLink | https://www.ncbi.nlm.nih.gov/pubmed/17069786$$D View this record in MEDLINE/PubMed |
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Copyright | 2006 The Canadian Society of Clinical Chemists |
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CorporateAuthor | on behalf of the National Institute of Child Health and Development (NICHD) Neonatal Research Network The Phototherapy Subcommittee National Institute of Child Health and Development (NICHD) Neonatal Research Network Phototherapy Subcommittee |
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Keywords | B f-100 kp B feq Bilirubin/albumin binding B f Cl K NRN A 460 B f-50 Peroxidase test Hyperbilirubinemia TBC Unbound bilirubin Newborn jaundice Free bilirubin B fss CPMC |
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Notes | ObjectType-Article-2 SourceType-Scholarly Journals-1 ObjectType-Undefined-1 ObjectType-Feature-3 content type line 23 Principal Investigator. NICHD Neonatal Research Network 2004: Alan Jobe, Neonatal Network Chair; Case Western Reserve University (U10 HD21364): Michele C. Walsh*, Nancy Newman; University of Cincinnati (U10 HD27853, M01 RR08084); Edward F. Donovan*, Cathy Grisby; Emory University (U10 HD27851, M01 RR00039): Barbara J. Stoll*, Ellen Hale; Indiana University (U10 HD27856, M01 RR00750): James A. Lemons*, Lucy Miller; University of Miami (U10 HD21397): Shahnaz Duara*, Ruth Everett; University of Alabama (U10 HD34216): Waldemar A. Carlo*, Monica Collins; Stanford University (U10 HD27880, M01 RR0070): David K. Stevenson*, M. Bethany Ball; University of Texas at Houston (U10 HD21373): Jon E. Tyson*, Georgia McDavid; University of Texas Southwestern Medical Center at Dallas (U10 HD40689): Walid Salhab*, Abbot R. Laptook*, Gaynelle Hensley; Wayne State University (U10 HD21385): Seetha Shankaran*, Rebecca Bara; Women and Infants’ Hospital (U10 HD27904): William Oh*, Angelita Hensmann; Yale University (U10 HD27871, M01 RR00125): Richard Ehrenkranz*, Pat Gettner; University of California at San Diego (U10 HD40461): Neil N. Finer*, Wade Rich; Duke University (U10 HD40492): C. Michael Cotton*, Kathy Auten; University of Rochester (U10 HD40521, M01 RR00044): Dale L. Phelps*, Linda Reubens; Wake Forest University (U10 HD40498): Lisa K. Washburn*, Nancy Peters; National Institute of Child Health and Human Development: Rosemary D. Higgins*; Research Triangle Institute (U01 HD36790): W. Kenneth Poole*, Abhik Das, Kristin Zaterka-Baxter, Betty Hastings, Carolyn Petrie. Corresponding Author: Charles E. Ahlfors, M.D. PO Box 2904 Vashon, WA 98070 Phone: 206-567-0599 Fax: 650-724-2103 E-mail: Ligand@centurytel.net Subcommittee Members: William Oh, Brown University, Providence, RI; Jon E. Tyson, University of Texas, Medical School at Houston, Houston, TX; Dale Phelps, University of Rochester, Rochester, NY; Michael O’Shea, Wake Forest School of Medicine, Winston Salem, NC; Kenneth Poole, Research Triangle Institute, Research Triangle Park, NC; Linda L. Wright, National Institute of Child Health and Development, Rockville, MD |
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Snippet | To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl
−) on plasma unbound bilirubin (
B
f) measurements made using a... To assess the effects of sample dilution, peroxidase concentration, and chloride ion (Cl(-)) on plasma unbound bilirubin (B(f)) measurements made using a... |
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SubjectTerms | Analytic Sample Preparation Methods Bilirubin - blood Bilirubin/albumin binding Chlorides - chemistry Diagnostic Techniques and Procedures - instrumentation Diagnostic Techniques and Procedures - standards Female Free bilirubin Humans Hyperbilirubinemia Infant, Newborn Infant, Premature - blood Jaundice, Neonatal - diagnosis Newborn jaundice Peroxidase test Peroxidases - chemistry Unbound bilirubin |
Title | Effects of sample dilution, peroxidase concentration, and chloride ion on the measurement of unbound bilirubin in premature newborns |
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