Development and Evaluation of a Chromatographic Procedure for Partial Purification of Substance P with Quantitation by an Enzyme Immunoassay

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Clinical and Diagnostic Laboratory Immunology, May 1998, p. 303-307, Vol. 5, No. 3
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Development and Evaluation of a Chromatographic Procedure for Partial Purification of Substance P with Quantitation by an Enzyme Immunoassay

William P. Fehder,¹^, Wen-Zhe Ho,²^,³ Donald E. Campbell,¹^,²^,³ Wallace W. Tourtellotte,⁴ Lisa Michaels,¹ Joann R. Cutilli,² Marina Uvaydova,² and Steven D. Douglas¹^,²^,³^,^*

Division of Immunologic and Infectious Diseases, Department of Pediatrics, University of Pennsylvania School of Medicine,¹ Joseph Stokes Jr. Research Institute,² and Clinical Immunology Laboratories, Children's Hospital of Philadelphia,³ Philadelphia, Pennsylvania, and Multiple Sclerosis Human Neurospecimen Bank, Veterans Affairs Medical Center, Los Angeles, California⁴

Received 15 October 1997/Returned for modification 15 December 1997/Accepted 21 January 1998

We have developed a simple chromatographic procedure for the partial purification of substance P (SP) from acidified plasmaand serum samples. We have evaluated a sensitive antigen competitionenzyme immunoassay (EIA) for the quantitation of SP. The chromatographicprocedure has recovery efficiencies ranging from 94.8 to 125%.The immunoreactivity of unknown amounts of purified SP subjectedto the preparative procedure yielded a coefficient of varianceof 9.4%. The EIA yielded reproducible standard curves having aninterassay (n = 8) correlation coefficient of 0.984. The evaluationof normal adult control serum yielded a mean value of 51 pg/ml(range, 35 to 61 pg/ml). The evaluation of 3.33× concentratesof serum-derived partially purified SP provided uncorrected SPvalues of 117 to 201 pg/ml, which fell within the midpoint ofthe three-decalog standard curve. These studies indicate thatboth the preparative and quantitative procedures are requiredfor the detection of SP in plasma or serum samples collected frompatients with several clinical disorders.

^* Corresponding author. Mailing address: Division of Infectious Diseases and Immunology, Children's Hospital of Philadelphia,34th St. and Civic Center Blvd., Philadelphia, PA 19104. Phone:(215) 590-2353. Fax: (215) 590-3044. E-mail: douglas{at}email.chop.edu.

Present address: School of Nursing, Allegheny University of The Health Sciences, Philadelphia, Pa.

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