Detection of antibodies directed at M. hyorhinis p37 in the serum of men with newly diagnosed prostate cancer

After Institutional Review Board approval and signed informed consent, serum samples were prospectively collected from 321 men presenting to the Department of Urology University of Florida for evaluation of BPH or prostate cancer from 2006-2009. Briefly, 5-ml of whole blood was collected in a serum separating tube from each subject. Within 30 minutes, the tube was placed in the centrifuge and spun for 15 minutes at 2400 rpm as dictated in our standard operating procedures of our departmental tissue bank. Fifty microliter of serum was pipetted into multiple 1-ml cryogenic vials, snap-frozen and stored at -80°C for future use. Hospital records were reviewed for demographic, clinical and pathologic data. A total of 219 subjects (N = 114, BPH and N = 105, prostate cancer) with adequate hospital records and banked serum samples comprised the study cohort.

M. hyorhinis p37 (MH38-113) was expressed and purified as previously described [16]. Briefly, plasmids were transformed into BL21(DE3)pLysS E. coli cells. The transformation was used to inoculate 1-L LB media with 100 mg L21 ampicillin and cultured at 37°C until the OD 600 nm was 0.7-1.0. Cells were induced using 1 mL of 1M isopropyl b-D-1 thiogalactopyranoside and allowed to express for three hours. Cells were lysed by vortexing the pellet in 1/10 the original volume of 20 mmol/L phosphate buffer (pH 7.8) followed by a sonication for three 15-second cycles. The resulting crude cell lysate was centrifuged at 40,000 × g for 20 minutes at 4°C to remove cell debris. The clear supernatant (soluble cellular extract) was subjected to ion exchange chromatography using the Econo System (Bio-Rad). A 5 mL Bio-Rad Econo-Pac S cation exchange column was attached to the bottom of a 50 mL Bio-Rad anion exchange Q column, and equilibrated with 20 mmol/L sodium phosphate buffer (pH 7.95) at a flow rate of 2.5 mL/min. Approximately 125 mg of soluble cellular extract were loaded on the column. The flow-through containing M. hyorhinis p37 was adjusted to pH 6.1 with 2 mol/L acetic acid, and loaded on a 5 mL cation exchanger, Bio-Rad Econo-Pac S cartridge, equilibrated with 20 mmol/L sodium acetate, pH 6.1 (buffer A). The column was washed with 5% buffer B [20 mmol/L sodium acetate (pH 6.1), 1 mol/L NaCl] and the M. hyorhinis p37 protein was eluted with 15% buffer B. The eluted sample was then concentrated using a Centriprep 10 spin column (Millipore, Bedford MA). Purity was confirmed by 10% SDS-PAGE stained with Coomassie Blue (Figure 1). Concentrations were calculated by absorbance at 280 nm using a calculated extinction coefficient of 54,620 M^-1cm^-1.

We used a naturally occurring antibody as an internal control. The disaccharide, Gal1α1,3 Gal, is present in all humans, and IgG antibodies to Gal1α1,3 Gal are found to be present in high titers in the serum of every normal individual, and are constantly produced throughout life [21]. Gal1α1,3 Gal was purchased from Sigma Chemical Co., St. Louis, Missouri, USA. Test serum samples were also assayed with Galα1,3 Gal as the substrate (positive control) coupled to bovine serum albumin (BSA). BSA alone served as the negative control. Plates were read at 405 nm in a plate reader. All of the sera tested showed a strong positive response against Galα1,3 Gal-BSA and no response to BSA alone (data not shown).

We used the Wilcoxon rank-sum test to compare the O.D. values and PSA values in the prostate cancer group to those in the BPH group. Since we are testing the hypothesis that the O.D. values and PSA values in the prostate cancer group are higher than that in the BPH group, all reported p-values are one-sided. The one-sided Wilcoxon rank-sum test is also used to assess the correlation between O.D. values and clinical parameters. We defined a diagnostic test (positive indirect ELISA assay vs. negative indirect ELISA assay) using a cutoff value of O.D. selected to maximize the sum of the sensitivity and specificity of the test [22]. All data analyses were performed using SAS software version 9.1.3.