Molecular characterization and expression of p23 (OspC) from a North American strain of Borrelia burgdorferi.

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Infect Immun. 1993 December; 61(12): 5097-5105

Molecular characterization and expression of p23 (OspC) from a North American strain of Borrelia burgdorferi.

S J Padula, A Sampieri, F Dias, A Szczepanski and R W Ryan

Department of Medicine, University of Connecticut Health Center, Farmington 06030-1310.

ABSTRACT

We have found that sera from patients with early stages of Lymedisease contain predominant immunoglobulin M reactivity to amajor 23-kDa protein (p23) from Borrelia burgdorferi 2591 isolatedin Connecticut. To characterize this immunodominant antigen,we cloned and sequenced p23 and found it to be 83% identicalby nucleotide sequence and 75% identical by amino acid sequencedto pC (recently renamed OspC), an abundantly expressed proteinon the outer surface of PKo, a European strain of B. burgdorferi(B. Wilske, V. Preac-Mursic, S. Jauris, A. Hofmann, I. Pradel,E. Soutschek, E.Schwab, G. Will, and G. Wanner, Infect. Immun.61:2182-2191, 1993). In addition, immunoelectron microscopylocalized p23 to the outer membrane, confirming that p23 isthe strain 2591 homolog of OspC. The North American strain B31,commonly used in serologic assays for Lyme disease, does notexpress OspC. Northern (RNA) blot analysis detected low levelsof ospC mRNA in B31, and DNA sequencing of the ospC gene fromB31 revealed a 54-bp deletion in the upstream regulatory region,possibly accounting for the low transcriptional activity ofospC. The ospC coding region from B31 was cloned and antibody-reactiveOspC was expressed in Escherichia coli. An immunoglobulin Menzyme-linked immunosorbent assay using recombinant OspC asthe target antigen shows promise for the serodiagnosis of earlystages of Lyme disease.

Infect Immun. 1993 December; 61(12): 5097-5105

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