Factor H in Porcine Seminal Plasma Protects Sperm against Complement Attack in Genital Tracts*

We found that factor H (FH) exists in porcine seminal plasma. Purified FH strongly inhibited serum alternative pathway complement activation against lipopolysaccharide. The molecular weight, pI, and heparin-binding activity of the purified protein were different from those of purified FH from porcine serum. The complement regulatory activity of seminal plasma FH was ∼2-fold stronger than that of serum FH. Treatment of purified serum FH with sialidase and N-glycosidase F gave almost the same results as those of seminal plasma FH. The deletion of sialic acid from the carbohydrate chains of both FHs contributed to heparin-binding and complement regulatory activities. Results of reverse transcriptase-PCR, Western blot analysis, and immunohistochemistry showed that seminal plasma FH is mainly secreted from epithelial cells of the seminal vesicle in male genital tracts. FH was also detected in the outer acrosomal region of ejaculated sperm by immunofluorescence staining, and found that the purified FH from the sperm membrane has the same complement regulatory activity as that of seminal plasma FH. The ejaculated sperm possessing FH in the outer acrosomal region considerably evaded complement attack. We also found that there is strong complement activity in fluids from female genital tract ducts. These findings indicate that FH bound to the outer acrosomal region and soluble FH play important roles in protecting sperm against complement attack in male and female genital tracts.

anti-mouse IgG horseradish peroxidase-linked whole antibody were obtained from GE Healthcare. Matrex Gel Red A was purchased from Amicon (Lexington, MA). Mouse polyclonal anti-C5b-9 antibody was purchased from Abcam (Cambridge, UK). Histofine (SAB-Po kit) was purchased from Nichirei Co. Ltd. (Tokyo, Japan). TRIzol reagent and Alexa Fluor 488 goat antirabbit IgG were purchased from Invitrogen. Transcriptor Firststrand cDNA Synthesis Kit and Taq DNA polymerase were products of Roche Diagnostics. Polyvinylidene difluoride membranes were purchased from Bio-Rad. Bacterial lipopolysaccharide (LPS) was purchased from Sigma. Mouse antiporcine CD46 antibody (6D8/9) was obtained from Serotec (Oxford, United Kingdom).
Polyacrylamide Gel Electrophoresis-Slab gel electrophoresis was carried out on 12.5% polyacrylamide gels according to the method described by Laemmli (27). Proteins in the gel were stained with Coomassie Brilliant Blue R-250.
Purification of FH from PSP-All purification steps were performed at 4°C unless otherwise specified, and 1 mM EDTA and phenylmethylsulfonyl fluoride were added to all buffers. PSP (ϳ500 ml) was dialyzed overnight against 20 mM Tris-HCl buffer, pH 7.5. The dialysate was centrifuged at 8,000 ϫ g for 45 min to remove the precipitate. The supernatant was applied onto a Q-Sepharose column (6 ϫ 10 cm) equilibrated with 20 mM Tris-HCl buffer, pH 7.5. After extensively washing the column with equilibration buffer, the proteins were eluated with a linear gradient from 0 to 0.5 M NaCl. Fractions containing FH activity were collected and concentrated with solid ammonium sulfate (80% saturation). The precipitate was dissolved in a minimum volume of 20 mM phosphate buffer, pH 6.8, and dialyzed overnight against the same buffer.
The dialysate was applied onto a Matrex Gel Red A column (2.5 ϫ 20 cm) equilibrated with 20 mM phosphate buffer, pH 6.8, and these fractions containing FH activity were collected. The fraction was dialyzed overnight against 20 mM phosphatebuffered saline, pH 8.0. The dialysate was applied at a flow rate of 0.4 ml/min onto a Superdex 200 pg column (2.6 ϫ 60 cm) equilibrated with the above buffer in fast protein liquid chromatography system. The FH fraction was collected and dialyzed overnight against PBS. The sample solution was used in subsequent experiments. FH concentration was determined by the single radial immunodiffusion method as described by Mancini et al. (28).
Preparation of Anti-FH Antibody and Immunoaffinity Column-Purified FH from PSP was used to raise a polyclonal antibody against rabbits. Briefly, 150 g of purified FH in 20 mM Tris-HCl buffer containing 0.15 M NaCl, pH 7.5, was used for the initial injection, and then five booster injections were given every 10 days. For initial injection, the antigen solution was mixed with an equal volume of complete adjuvant, and incomplete adjuvant was used for subsequent injections. Antibody preparation was carried out at the Research Center for Animal Life Science of Shiga University of Medical Science under the institutional guidelines for animal use. The antisera were collected, and anti-FH antibody was purified from antisera using an FH ligand column. Purified anti-FH antibody was used for immunohistochemical staining, immunoblot analysis, and preparation of an immunoaffinity column. Purified antibody (7.5 mg) was coupled to a CNBr-activated Sepharose 4B (GE Healthcare) according to the manufacturer's instructions.
Determination of N-terminal Amino Acid Sequence-The purified FH was subjected to 10% SDS-PAGE, and the protein on the gel was blotted onto a polyvinylidene difluoride membrane. The protein bands on the membrane were cut out and sequenced using an Applied Biosystems Model 492cLC Protein Sequencer equipped with an online phenylthiohydantoin analyzer (ABI 140D Microgradient Delivery System, Foster City, CA).
Deglycosylation of FH by PNGase F-The N-linked glycans of the purified FH from PSP and PS (porcine serum) were removed with N-glycosidase F (PNGase F, Enzymic In-solution N-Deglycosylation kit) under reducing and denaturing conditions according to the instructions of the manufacturer (Sigma). Briefly, 40 g of freeze-dried FH was resuspended in 90 l of reaction buffer. FH was further denatured by addition of octyl ␤-D-glucopyranoside and ␤-ME and then incubation at 100°C for 10 min. After adding a protease inhibitor mixture (Calbiochem) and 5 l of PNGase F solution (500 units/ml), the mixture was incubated at 37°C overnight. After boiling, the sample was subjected to SDS-PAGE analysis followed by staining with Coomassie Blue. Furthermore, PNGase F-treated PS FH for the complement regulatory assay was prepared under nondenaturing conditions.
Sialidase Treatment of FH from PS-The sialic acid of the purified PS FH was removed by sialidase treatment. About 1 mg of freeze-dried PS FH was suspended in 1 ml of 0.1 M sodium acetate buffer, pH 5.5, containing 4 mM CaCl 2 . After adding protease inhibitors (Complete Mini EDTA-free, Roche) and 100 l of sialidase solution (type VIII, Sigma, 10 units/ml), the mixture was incubated at 37°C overnight. Sialidase-treated PS FH was then purified by heparin-affinity column chromatography and used for complement regulatory assay.
Determination of AP Complement Activity by Enzyme-linked Immunosorbent Assay-PS diluted in EGTA/gelatin veronal buffer (VBS containing 10 mM EGTA, 0.05% Tween 20, and 0.1% gelatin, pH 7.5) was preincubated in LPS-coated microtiter plates (Maxisorp, Nunc, Roskille, Denmark) for 5 min at 37°C. MgCl 2 was then added at a final concentration of 5 mM before incubation for 1 h at 37°C. Complement activity was assessed using a monoclonal antibody to direct membrane attack complex, followed by detection of the monoclonal antibody binding using horseradish peroxidase-conjugated anti-mouse IgG antibodies. ABTS (2,2Ј-azino-bis(3-ethylbenzthiazoline-6-sulfonic acid), Roche) substrate (absorbance at 405 nm) was used to estimate the presence of peroxidase antibodies. The absorbance was measured using a plate reader (Multiscan JX, Thermo Lab Systems, Yokohama, Japan). In the cases of determination of the complement regulatory activities of PS FH and PSP FH on AP, the percent purities of FHs used were Ͼ98% as judged by SDS-PAGE.
Isolation of RNA, cDNA Library Synthesis, and RT-PCR-Total RNA was isolated from porcine testis, epididymis caput, epididymis corpus, epididymis cauda, prostate, seminal vesicle, and liver using a High Pure RNA tissue kit (Roche) according to the manufacturer's recommendations. Reverse transcription was performed for 30 min at 42°C using Superscript II reverse transcriptase (Invitrogen), oligo(dT) primer, and 5 g of total RNA. PCR analysis was performed using 1 l of first strand cDNA as a template or 1 l of total RNA in RT-minus control reaction as a control with a 2720 thermal cycler (Applied Biosystems). Primers used for amplification were as follows: 5Ј-GAA AAA ATT CCA TGT TCT GA-3Ј (SCR15-20-F) and 5Ј-TCC ACA CGT AGG ATA GGC CA-3Ј (SCR15-20-R) for FH, and 5Ј-CCG TGG GTT GTT AAC TTG CC-3Ј (␤-actin-F) and 5Ј-CTG CAG CAC TTT ATT TCC TC-3Ј (␤-actin-R) for ␤-actin primers. PCR products were resolved on 1% agarose gels.
Immunohistochemical Staining of Various Porcine Genital Tract Tissues-Most of the adult porcine genital tract tissues including the testis, epididymis, seminal vesicle, and prostate were obtained within 5 min after anesthetic death by sodium pentobarbital. The tissue specimens were fixed in 10% neutral buffered formalin and embedded in paraffin and then cut into 5-m thick sections. Immunohistochemical staining of these tissue sections was carried out as described previously (29), and their images were taken using a Nikon Microphot FXA microscope (Tokyo, Japan).
Immunofluorescence Staining of Testicular, Epididymal, and Ejaculated Sperm-Spermatozoa were collected from the testis, epididymis, and ejaculated fluids and washed three times with PBS. The pellets supported on an aminopropyltriethoxysilanecoated slide glass (Matsunami Glass, Osaka, Japan) were fixed with methyl alcohol for 1 h at room temperature. After blocking with PBS containing 1% bovine serum albumin (1% bovine serum albumin-PBS), the specimen was reacted with 1:1000 diluted anti-FH antibody in 1% bovine serum albumin-PBS for 1 h at room temperature and then washed several times with PBS followed by incubation with 1:1000 diluted Alexa Fluor 488-conjugated goat anti-rabbit IgG antibody (Invitrogen) in 1% bovine serum albumin-PBS for 1 h at room temperature. After washing three times with PBS, sperm were coverslipped with Vectashield and 4Ј,6-diamidino-2-phenylindole (Vector Laboratories, Burlingame, CA). Each specimen was observed under an inverted fluorescent microscope (Olympus, Tokyo, Japan).
Purification of FH from Ejaculated Sperm Membrane-Ejaculated sperm (9 ϫ 10 8 ) were washed three times with PBS. Washed sperm were mixed with PBS containing 2% sodium cholate (Dojindo Laboratories, Kumamoto, Japan) and rotated for 15 min at 4°C. The mixture containing sperm was centri-fuged at 7,000 ϫ g for 30 min. The supernatant was applied onto an FH immunoaffinity column. The column was washed with PBS containing 2% sodium cholate and then washed with PBS containing 0.5 M NaCl. FH was eluted with 0.1 M glycine-HCl buffer, pH 3.0, and fractions were immediately neutralized to pH 7.5 with 1 M Tris-HCl buffer, pH 9.0.
Determination of AP Complement Activity on Epididymal and Ejaculated Sperm-Ejaculated and epididymis cauda sperm (2.4 ϫ 10 5 ) washed with PBS were coated overnight on a 96-well immunoplate. Nonspecific binding was blocked with PBS containing 0.1% porcine serum albumin. PS diluted with gelatin veronal buffer/EGTA without Tween 20 was put into each of the wells coated with sperm. AP complement activation and detection of complement binding were performed as described above.

Detection of AP Complement Activities in Fluids from Male and Female Genital Tracts and Seminal
Plasma-Fluids from the epididymis caput, corpus, and cauda, and seminal plasma in the porcine genital tract ducts and the fluids from porcine female genital tract ducts such as the vagina, uterus, corunu uterus, and ovary in the non-mating stage (season) were separately obtained from one institute and two local slaughterhouses with their courtesy. AP complement activity assay was carried out as described above.

FH Purification and Molecular Weight of the Purified FH-
FH was purified from ϳ500 ml of PSP by Q-Sepharose, Matrex Red A, and Superdex 200 pg (in fast protein liquid chromatography) columns. Table 1 shows representative results. The protein was purified ϳ274-fold with a 22.0% yield over the dialysis fraction. As shown in Fig. 1B, complement regulatory activities were detected in fractions F, G, and H and PSP FH as a protein was contained in these fractions (Fig. 1A).
The purified FH at the final step migrated as a single band on SDS-PAGE in the presence or absence of ␤-ME (Fig. 2). The overall yield of FH was ϳ6.7 mg from 500 ml of PSP. The molecular weights (M r ) of the purified protein were 140,000 in the absence and 155,000 in the presence of ␤-ME on 10.5% SDS-PAGE. The concentration of FH in PSP and PS was determined to be 14.8 and 58.6 mg/100 ml, respectively, by the single radial immunodiffusion method (28).
Comparisons of Molecular Weight, pI, Heparin-binding Activity, and Complement Regulatory Activity of FHs from PSP and PS-We compared the molecular weight, pI, heparin-binding activity, and complement regulatory activity of FH from PSP with those of FH from PS. Molecular weight of the purified PS FH was 144,000, and the protein was 4 kDa larger than that of PSP FH on SDS-PAGE (Fig. 3A). The same result was obtained by Western blotting and immunoprecipitation with affinity purified anti-FH antibody from PS and PSP (data not shown). As shown in Fig. 3B, deglycosylation of both FHs by PNGase treatment showed that both FHs migrated to the same position on SDS-PAGE. Furthermore, pI values of PSP FH and PS FH were 6.90 and 6.35, respectively, from two-dimensional electrophoresis (Fig. 3C). Comparison of the strengths of binding to a heparin column (Fig. 3D) showed that PSP FH bound to the column more strongly than PS FH. Complement regulatory activity of PSP FH against AP complement activation was 2-fold stronger than that of PS FH (Fig. 3E).
Effect of Glycosidase Treatment on Molecular Weight, pI, Heparin-binding Activity, and Complement Regulatory Activity of PS FH-To confirm the effect of carbohydrate chains containing sialic acid on heparin-binding and complement regulatory activities of PS FH, we compared those activities of non-treated PS FH with those of glycosidase-treated PS FH. M r values of PNGase F-treated PS FH and sialidase-treated PS FH were 140,000 and 142,000 (Fig. 4A), respectively. Sialidasetreated PS FH showed triple spots of pI values (6.92 (1), 6.82 (2), and 6.40 (3), respectively) in two-dimensional electrophoresis (Fig. 4B). Comparison of the strengths of binding to a heparin column (Fig.  4C) showed that sialidase-treated PS FH bound to the column more strongly than non-treated PS FH. Complement regulatory activities of PNGase and sialidase-treated PS FH against AP complement activation were 1.2-and 1.5-fold stronger, respectively, than that of nontreated PS FH (Fig. 4D).
Regulation of AP Complement Activation by FH-free PSP-FHfree PSP was prepared by passing PSP through an anti-FH immunoaffinity column. PSP was also passed through a Sepharose 4B column as a control.
There was a significant difference between complement regulatory activities of FH-free PSP and PSP (Fig. 5). The regulatory activity of PSP was significantly suppressed by removing FH.
Expression and Localization of FH Protein in Genital Tract Tissues-To determine the genital tract tissues in which FH was secreted and expressed, we performed immunohistochemical analysis of porcine genital tract tissues, including the testis, epididymis, seminal vesicle, and liver, with affinity purified anti-FH antibody. FH was strongly stained in epithelial cells of the seminal vesicle and its fluid (Fig. 6A), and was stained very faintly in interstitial cells of the testis but not in the prostate (data not shown).
Detection of FH protein was also performed by immunoblot analyses to confirm whether or not the immunohistochemical stained protein was FH. An ϳ140-kDa protein band was detected in the seminal vesicle and a 144-kDa protein band was detected in the liver using the affinity purified anti-porcine FH antibody (Fig. 6B). In the male genital tracts, the density of the band originating from the seminal vesicle was stronger than that in other tissues such as the testis, epididymis, and prostate.
Moreover, based on the fact that FH consists of 20 modules termed short consensus repeats (SCR), which are composed of 60 amino acid residues, RT-PCR of SCR15-20 was performed using total RNA preparations from the porcine testis, epididymis, prostate, and seminal vesicle. Amplified PCR products were detected in the male genital tract tissues except the prostate. Large quantities of PCR products were detected in the testis, epididymis caput, and seminal vesicle. Each product was a single band of 1,200 base pairs (Fig. 6C). Sequencing of the corresponding cDNAs indicated that they are identical to those reported previously (30) (accession number AJ278470). There is a discrepancy between the PCR product and FH protein to M and the pass-through fraction (PTF) were dialyzed extensively against Milli-Q water and freeze-dried. The dried-up proteins were dissolved with gelatin veronal buffer. The assay of complement regulatory activity was performed using LPS-coated microtiter plates. Complement activity is presented as percent of the control level, which was measured as the complement activity added to purified FH (250 g/well). Purified porcine albumin (250 g/well) was used as a negative control. Each value is the mean Ϯ S.E. from triplicate experiments. expression data. ␤-Actin was used as an internal control because of its abundant expression.
Localization of FH on Testicular, Epididymal Sperm, and Ejaculated Sperm Membrane-We performed immunofluorescence staining to determine the localization of FH on sperm obtained from testis, epididymis caput, corpus, and cauda, and ejaculated sperm.
It was found that FH exists on the ejaculated sperm (Fig. 7,  E-1 and E-2). The outer acrosomal region of the ejaculated sperm was strongly stained (Fig. 7, E-1 and E-2). Sperm in the testis, epididymis caput, corpus, and cauda were scarcely stained (Fig. 7, A-D). FH was not detected on ejaculated sperm in the absence of anti-FH antibody (data not shown).
Regulation of AP Complement Activation by Purified FH from Ejaculated Sperm-To investigate complement regulatory activity of FH on the ejaculated sperm membrane, we purified FH from ejaculated sperm by detergent extraction and by using immunoaffinity column. The overall yield of FH was ϳ435 g from 9.12 ϫ 10 8 ejaculated sperm, and the purified protein migrated as a single band at 140 kDa on SDS-PAGE (Fig. 8A). Purified FH from the ejaculated sperm membrane regulated the AP complement activation in a dose-dependent manner by 50% of the control level at the concentration of 10 g/100 l. There was no difference between the regulatory activities of FH originating from the sperm membrane and PSP FH (Fig. 8B).

Assessment of AP Complement Activity against Sperm from the Epididymis Cauda and Ejaculated
Sperm-We examined whether the ejaculated sperm are in fact able to evade the complement attack of AP in comparison with sperm from the epididymis cauda. Washed ejaculated sperm and sperm from the epididymis cauda were coated on 96-well immunoplates instead of LPS. Ejaculated sperm and sperm from the epididymis cauda evaded depositing membrane attack complex by 77 and 29% in comparison with that of the LPS level used as a positive control, respectively (Fig.  9). Membrane attack complex was not detected in the absence of sperm (data not shown). Fig. 10, AP complement activities were weakly detected in fluids from epididymis caput, corpus, and cauda, and seminal plasma. However, AP complement activities were detected more strongly (6 -10-fold) in fluids from some porcine female genital tract ducts such as the vagina, uterus, corunu uterus, and ovary in the non-mating stage (season) than in fluids from male genital tract ducts (Fig. 10). AP complement activities in fluids from male and female genital tract ducts including seminal plasma and ovaries were ϳ1:18 and 1:2 to 1:3 weaker, respectively, than that in serum (Fig. 10). Serum was used as a positive control.

DISCUSSION
Factor H is a regulatory protein of the AP. This protein, which possesses cofactor activity for factor I-mediated cleavage of C3b, competes with factor B in binding to C3b and decreases formation of the alternative pathway C3 convertase (C3bBb) (19,20). It has been reported that there are membraneassociated anti-complement proteins such as CD46 (MCP), CD55 (DAF), and CD59 in cell-free human and rat seminal plasma (31)(32)(33). However, a soluble type of anticomplement protein other than clusterin has not been identified in animal seminal plasma.
We tried to isolate FH from fresh PSP by column chromatographies on Q-Sepharose, Matrex Red A, and Superdex 200 pg. We also characterized its biochemical and biological properties and its role as a regulator in AP.
A typical procedure for purification of FH is summarized in Table 1. FH was finally purified 274-fold with a 22% yield over the dialyzed PSP. The overall yield of FH from ϳ500 ml of fresh PSP was ϳ6.7 mg. The concentration of FH in PSP determined by the single radial immunodiffusion method (28) was 14.8 mg/100 ml. This value is 1 ⁄ 4 less than the concentrations of porcine serum FH (58.6 mg/100 ml) and human serum FH (30 -60 mg/100 ml) previously reported (34). This purified protein gave a single band on SDS-PAGE in the absence and presence of ␤-ME (Fig. 2). The M r values of the purified FH were 140,000 and 155,000 on SDS-PAGE in the absence and presence of ␤-ME, respectively. On the other hand, M r values of FH purified from porcine serum were 144,000 and 159,000 on SDS-PAGE in the absence and presence of ␤-ME, respectively. pI values of the purified FHs from PSP and PS were 6.90 and 6.35, respectively, in two-dimensional electrophoresis. Although M r and pI values of the two purified FHs were different, the first N-terminal 20-amino acid sequences of the two FHs were identical. We also compared the inhibitory activity of purified seminal plasma FH with that of purified serum FH. The inhibitory activity of purified seminal plasma FH was stronger (about 2-fold) than that of purified serum FH (Fig. 3E). It has been reported that the N-terminal domain of FH plays an important role in regulation of complement activation and that the C-terminal domain of FH is mainly involved in binding to heparin (22,36). Therefore, we compared the heparin-binding activities of the two FHs. Heparin-binding activity of purified seminal plasma FH was stronger than that of serum FH, and both puri-  fied proteins after PNGase F treatment moved to the same molecular weight position on SDS-PAGE (Fig. 3B). Moreover, heparin-binding activity of sialidase-treated PS FH was stronger than that of non-treated PS FH (Fig. 4C). This result indicates that the differences in heparin-binding activity and pI are due to deletion of sialic acid at glycosylation sites in both FHs. On the other hand, complement regulatory activity of sialidasetreated PS FH was stronger than that of non-treated PS FH. A similar result was also obtained using PNGase F-treated PS FH (Fig. 4D). Therefore, the stronger regulatory activity of purified PSP FH indicates that PSP FH has truncated molecules at the carbohydrate chains including sialic acid and the steric hindrance of the carbohydrates affects the regulatory activity of both FHs. The deletion of sialic acid from the carbohydrate chains of PS FH is thought to contribute to its stronger complement regulatory activity. Generally, sialidase in human (or rat) seminal plasma releases bound sialic acid from the sperm membrane, thereby increasing the concentration of free sialic acid in human (or rat) seminal plasma (37). It has been reported that the concentration of sperm-bound sialic acid gradually decreases from the caput to the cauda epididymis during epididymal migration, and decreased sperm-bound sialic acid concentration contributes to elevation in sperm motility (38). Furthermore, comparison of PSP and FH-free PSP (Fig. 5) showed that the regulatory activity of PSP was significantly decreased by removing FH. These results suggest that FH plays an important role in regulation of complement activation of AP in seminal plasma. In humans and mice, it has been reported that Twenty-five g of each tissue was homogenated, and purified RNA was obtained as described under "Experimental Procedures." RT-PCR products were separated in 1.5% agarose. Lanes from left to right refer to mRNA from: testis, epididymis caput, epididymis corpus, epididymis cauda, prostate, seminal vesicle, and liver. ␤-Actin was used as an internal control. Liver was used as a positive control. FIGURE 7. Immunofluorescence staining of FH on the sperm membrane. Sperm obtained from the testis (A), epididymis caput (B), epididymis corpus (C), and epididymis cauda (D) and ejaculated sperm (E-1 and E-2) on a poly-Llysine-coated slide glass were fixed and stained with affinity purified anti-FH antibody followed by Alexa 488-conjugated goat anti-rabbit IgG. The outer acrosomal region of ejaculated sperm was strongly stained (green). The tails of sperm obtained from testis, epididymis caput, corpus, and cauda tissues were very faintly stained. Original magnifications: A-E-1, ϫ800, and E-2, ϫ200. Nuclei were stained with 4Ј,6-diamidino-2-phenylindole (blue).
seminal plasma has strong complement regulatory activity due to both MCP and DAF (30,31). These proteins with complement regulatory activity of an alternative pathway were expressed in the testis and prostate. The former is anchored on the inner acrosomal membrane of sperm and the latter is secreted from the prostate with glycosylphosphatidylinositol anchored on prostasome (39,40). It has been suggested that the role of prostasome is to transfer proteins to sperm (41). After ejaculation, these complement regulatory proteins are transferred to the sperm to protect against complement attack (42).
We attempted to identify the complement regulatory factor(s) against AP in PSP by fractionation of PSP using Q-Sepharose column chromatography. However, no inhibitory or regulatory protein peaks other than that of FH were detected (Fig. 1B).
It has been reported that 60-, 50 -55-, and 45-kDa bands of CD46 (MCP) were detected in human testicular tissue lysate and that the 45-kDa band was an inner acrosomal membrane anchoring protein and the 60-kDa band was a human prostasome-specific type protein (43). To evaluate tissue distribution of CD46, using an antibody against CD46, we determined the expression of the protein in porcine genital tract organs, seminal plasma, and sperm lysate. 60-and 45-kDa CD46 was identified in the testis, epididymis, prostate, and seminal vesicle. However, it was revealed that CD46 does not exist in seminal plasma and sperm lysate. CD46 was also not detected inmmunohistochemically in the sperm acrosomal membrane (data not shown). Accordingly, FH, but not CD46, CD55, or CD59, may play important roles in protection of sperm against complement attack of an alternative pathway in porcine genital tracts.
As shown in Fig. 6A, FH was also stained in epithelial cells and fluids of the seminal vesicle. Western blot and RT-PCR analyses also revealed that FH was synthesized in epithelial cells of the seminal vesicle (Fig. 6, B and C) and secreted into fluid of the seminal vesicle. However, it was found that there is a discrepancy between gene and protein expressions. The discrepancy indicates that there may be a translational disorder or degradation of nascent or synthesized FH after normal translation (44,45).  . Assessment of AP complement activation on the sperm membrane. AP complement assay was performed using a 96-well immunoplate coated with sperm from the epididymal cauda or ejaculated sperm. LPS was used as a positive control. Similar results were obtained from at least three separate experiments. Each value is the mean Ϯ S.D. from triplicate experiments. *, p Ͻ 0.001, ejaculated sperm were significant compared with epididymal sperms. FH was also found to be localized on ejaculated sperm membranes. To compare the regulatory activity of seminal plasma FH with that of sperm membrane FH, we tried to elute FH from sperm membranes with various reagents. Sperm membranebound FH was eluted in turn with 2% sodium cholate ϭ low pH (pH 3.0) Ͼ 2% Chaps Ͼ 2% octyl glycoside. However, phosphatidylinositol-phospholipase C, neuraminidase, and high ion strength such as 1 M NaCl could not release FH from sperm membrane. Accordingly, it is thought that FH binds to sperm membranes in a hydrophobic binding manner. Comparison of seminal plasma FH and FH eluted from sperm membranes showed that both FHs have the same M r and complement regulatory activities (Fig. 8). The ejaculated sperm showed ϳ3-fold stronger activity than that of the epididymal sperm for regulation of complement activation (Fig. 9). These results indicate that FH on the membrane of ejaculated sperm is able to directly inhibit complement activation. Furthermore, to confirm the function of PSP FH, we determined complement activity in fluids from several male and female genital tract ducts, seminal plasma, and ovary fluid. As shown in Fig. 10, complement activity was weakly detected in fluids from the porcine genital tract ducts and seminal plasma (35,46,47). However, the activities in secreted or transudatory fluids of female genital tract ducts were 6 -10-fold stronger than those in seminal plasma. This indicates that binding of FH to the sperm outer acrosomal region contributes to the decay of complement attack on sperm advancing into female genital tract ducts. It is therefore thought that these two types of FH play important roles in realization of fertilization in the porcine. Furthermore, the existence of soluble FH in seminal plasma is thought to contribute to self-protection against bacterial infections in the both male and female genital tracts.