Comparative studies on the binding specificities of pertussis toxin and different lectins to human erythrocytes

The binding specificity of pertussis toxin (PT) was compared with lectins with well-defined specificities by hemagglutination, hemagglutination inhibition and competitive binding assays. Neuraminidase-treated human erythrocytes were much less weakly agglutinated by PT than untreated ones. Hemagglutination of untreated human type A erythrocytes by PT was inhibited by fetuin, haptoglobulin and hog A + H. Mono- and disaccharides, and N-acetylneuraminic acid alone were ineffective at the highest concentrations used. On the other hand, hemagglutination by Ricinus communis agglutinin (RCA-1) was effectively inhibited by these substances. Similar results were also obtained in competitive binding assays with 123I-labeled PT and untreated type A erythrocytes. The binding of 125I-labeled PT to type A erythrocytes was not effectively inhibited by any of lectins with well-defined specificities. These results suggest that the combining site of PT may be specific for terminal sialic acid and/or sialic acid-linked carbohydrate portion(s) which can not be recognized by lectins reported previously.     

Characterization of the interaction between VP8 of bovine rotavirus C486 and cellular components on MA-104 cells and erythrocytes.

Rotavirus VP8*, the N-terminal trypsin cleavage product of VP4, has been shown to bind to MA-104 cells and human O type erythrocytes. To examine whether bacterially expressed VP8* binds to cellular components of MA-104 cells, the VP8* (aa 1-247) was expressed in E. coli and radiolabelled with 35S-methionine. The radiolabelled rVP8* was immunoprecipitated with antiserum to bovine rotavirus C486 (BRV). The rVP8* was found to bind to MA-104 cells and its binding was competed by BRV. To study the interaction between VP8* and receptors of erythrocytes, hemagglutination (HA) and hemagglutination inhibition (HI) assays were carried out using solubilized rVP8*. rVP8* showed HA which could be inhibited by antiserum to BRV. This interaction was also inhibited by gangliosides, demonstrating a sialic acid dependent interaction. To study the contribution of the C-terminal region of VP8* to HA, a number of approaches were used. First, a peptide spanning aa 230-247 was synthesized and antisera was raised against the peptide to see whether it could inhibit HA of rVP8*. Second, a truncated form of VP8* (tVP8*: aa 1-229) was expressed to examine its hemagglutinating activity. Third, the dimerization of rVP8* and tVP8* was compared by Western-blotting following electrophoresis using native SDS-PAGE. The results indicated that antibody to aa 230-247 inhibits hemagglutination by preventing dimerization of VP8* which in turn allows the molecule to cause HA. To characterize the interaction between the HA domain and sialic acid receptors, erythrocytes were treated with sialidases of different specificities. Arthrobacter ureafaciens, Clostridium perfringens and alpha 2-8 linkage-specific neuraminidase destroyed the ability of sialic acid of erythrocytes to interact with rVP8*, indicating that bovine rotavirus C486 binding requires an alpha 2-8 linkage but acetylation of the sialic acid is not necessary.     

The hemagglutinating activity of Pseudomonas aeruginosa strains isolated from humans and animals

The presence and type of adhesins occurring in Pseudomonas aeruginosa strains were determined by hemagglutination test with a 3% suspension of normal and trypsin-treated human group A erythrocytes, with or without the addition of sugar inhibitors (D-mannose, D-glucose, L-fucose, D-galactose, D-fructose, lactose, N-acetylneuraminic acid, N-acetylglucosamine and N-acetylgalactosamine). This study showed that a low percentage of Pseudomonas aeruginosa strains caused the agglutination of normal erythrocytes. Trypsin treatment of erythrocytes did not affect the hemagglutinating properties, indicating that hemagglutination was not dependent upon a trypsin-sensitive protein on the erythrocytes surface. Most of the studied strains agglutinated RBCs at 37 degrees C. A great variability in the inhibiting activity on studied strains was observed among the carbohydrates tested. These results demonstrated the predominant role of N-acetylglucosamine, N-acetylgalactosamine and N-acetylneuraminic acid for Pseudomonas aeruginosa adhesion to RBCs.     

Serotype, hemolysin production, and adherence characteristics of strains of Escherichia coli causing urinary tract infection in dogs.

Virulence factors were studied in 82 strains of Escherichia coli isolated from the urine of dogs with urinary tract infections. The most frequently expressed O antigens were 2, 4, 6, 25, and 22/83. Most strains were K nontypeable. Mannose-sensitive hemagglutination (MSH) with canine erythrocytes was observed in 71 strains and mannose-resistant hemagglutination (MRH) was observed in 32 strains. Strains that caused MSH of erythrocytes from dogs also caused MSH of erythrocytes from guinea pigs. Most strains that caused MRH of human A1P1 erythrocytes also reacted with erythrocytes of dogs. Of 22 strains (27%) that agglutinated human A1P1 erythrocytes, but not A1p erythrocytes, 17 (77%) had specificity for globo A, but did not react with the galactose alpha 1----4galactose beta disaccharide receptor. The remaining 5 strains and 2 others that simultaneously expressed an X adhesin agglutinated galactose alpha 1----4galactose beta-coated latex beads. Bacterial adherence to canine uroepithelial cells from the bladder was most often observed in strains expressing MSH, less often observed in strains expressing MRH, and least often observed in strains that failed to induce hemagglutination. Adherence of MSH strains to canine uroepithelial cells was inhibited by alpha-methyl-D-mannoside. As a group, MRH strains expressing globo-A- and galactose alpha 1----4galactose beta-specific adhesins did not have strong adherence. Strains of E coli isolated from dogs with urinary tract infections most commonly expressed type-1 fimbriae, and the main mechanism of in vitro adherence to canine uroepithelial cells involved a mannose-sensitive mechanism. Overrepresentation of globo-A-specific adhesins did not appear to be related to adherence of canine uroepithelial cells.     

Lectin binding and the carbohydrate moieties present on Newcastle disease virus strains

Lectin-binding profiles were developed for 14 strains of Newcastle disease virus in order to determine the carbohydrate moieties associated with hemagglutination and to establish whether there are any associations between the carbohydrates present on the virus envelope and virulence. All strains of Newcastle disease virus were bound by concanavalin A. Other lectins bound the viruses differentially, but there was no pattern of binding that could be associated with viral virulence. The binding of virus by Lens culinaris lectin was associated with the elution rate of the virus from chicken erythrocytes. Strains that elute rapidly from chicken erythrocytes were not bound by Lens culinaris lectin. The sugar alpha-D-N-acetylglucosamine inhibited the adsorption of Lens culinaris lectin to the strains that were "slow eluters" from chicken erythrocytes.     

Hemagglutination by calf diarrhea coronavirus

The virus was grown in BEK-1 cells, a stable cell line from bovine embryo kidney, and tested for hemagglutination (HA) with erythrocytes of a variety of species at 4°C, room temperature and 37°C. HA was observed at all temperatures with chicken, mouse, rat, and hamster erythrocytes but not with erthyrocytes of human (O), cattle, horses, sheep, guinea pigs, geese, ducks, pigeons and 1-day-old chicks. Chickens showed an individual variation in agglutinability of their erythrocytes, requiring selection of birds to obtain erythrocytes for HA. HA reaction was inhibited by specific antiserum. Some factors involved in HA and HA inhibition (HI) were investigated and standard HA and HI tests were worked out.     

Hemagglutination and antigenic comparison of rabbit hemorrhagic disease virus

The hemagglutinating activity and serological properties of three strains of rabbit hemorrhagic disease virus, Chinese, Korean and Shizuoka, which was first isolated in Japan, were examined by hemagglutination (HA) and cross hemagglutination inhibition (HI) test with human erythrocytes. Similar results were observed between the Chinese and Korean strains, both of which gave positive HA at 4 degrees C with O, A, B and AB, and at 22 degrees C with B and AB blood groups. In the Shizuoka strain, positive HA was observed at 4 degrees C with O, A, B and AB, at 22 degrees C with A, B And AB, and at 37 degrees C with B blood group. In experimentally infected rabbits, HI antibody in these animals showed a titer of 16,384 or 32,768 at 4 weeks after inoculation. No serological difference was observed in three strains by cross HI test.     

Recombinant galectins of male and female Haemonchus contortus do not hemagglutinate erythrocytes of their natural host

Recombinant galectins of female and male adult worms of Haemonchus contortus were expressed in Escherichia coli and their hemagglutinating activities to human and different animal erythrocytes were analyzed. The results showed that female and male galectins could be highly expressed in E. coli using a temperature-sensitive plasmid, with the recombinant protein being mainly appeared in inclusion bodies. Hemagglutinating activity assays showed that both of the galectins hemagglutinated human A, B, O type, dog, rabbit, chicken and mouse erythrocytes at the high concentration of 40 microg/well, but did not hemagglutinate erythrocytes of the natural host of H. contortus, the goat. Sugar inhibition assays confirmed that, out of eight sugars tested, only lactose was effective to inhibit agglutination of human type B erythrocytes by the recombinant galectins.     

Identification of possible chicken intestinal mucosa receptors for SEF21-fimbriated Salmonella enterica serovar Enteritidis

In order to test whether glycosphingolipids (GSLs) on the chicken intestinal mucosa serve as a receptor for Salmonella enterica serovar Enteritidis with fimbriae, we analyzed neutral GSLs and gangliosides from chicken intestinal mucosa and investigated the binding of bacteria to neutral GSLs and gangliosides. Four kinds of neutral GSLs, designated as N-1 to N-4 and four kinds of gangliosides, named G-1 to G-4, were identified on high-performance thin-layer chromatography (HPTLC) plates. In TLC immunostaining tests, fimbriated S. Enteritidis bound only to glucosylceramide (GlcCer) standard, N-1, GM3 standard and G-1, but neither to N-2, N-3, N-4, nor to G-2, G-3 and G-4. Further, the bacterial binding to N-1 and G-1 was completely inhibited by preincubation of bacteria with anti-S. Enteritidis fimbriae (SEF) 21 antibody, but not by anti-SEF14 antibody. These results suggest that both GlcCer (N-1) and ganglioside GM3 (G-1) on the epithelial cell surfaces of chicken intestine act as receptors for fimbriated S. Enteritidis.     

对FC株猪源性肠毒素型大肠杆菌致病因子的研究

FC菌株是一株从腹泻仔猪粪便中分离的肠毒素型大肠杆菌(Enterotoxigenic E.coli,ETEC)。在MRHA反应中,本菌能凝集人O型、豚鼠、马、绵羊、牛、鸡和兔的红细胞,对人O型和豚鼠红细胞有很高的血凝性,血抗K88和K99血清不能抑制其对豚鼠和绵羊红细胞的血凝。在体外小肠上皮细胞吸附试验中,本菌对仔猪小肠上皮细胞具有强烈的吸附作用;透射电镜和扫描电镜观察证实了FC株菌除表面具有一种纤毛样结构外,还能定居在仔猪小肠段。血清学试验结果表明,本菌的O抗原属于O101。K88和987P两种抗血清均不能凝集本菌,而K99和F41抗血清均可凝集。对纯化的FC株菌粘着素抗原作等电聚焦和聚丙烯酰胺凝胶电泳分析,结果表明,该菌的粘着素是由等电点分别为4.61和9.78,分子量分别为29500和17500的两种蛋白质抗原所组成。此外,用乳鼠胃内投服试验和兔肠结扎试验证明,该菌只产生热稳定肠毒素。总之,本菌是一株能产生ST的K99,F41的肠毒素型大肠杆菌。     

Antigenic variant of swine influenza virus causing proliferative and necrotizing pneumonia in pigs.

A new antigenic variant of swine influenza virus was isolated from the lungs of pigs experiencing respiratory problems in 7 different swine herds in Quebec. Pigs of different ages were affected, and the main clinical signs were fever, dyspnea, and abdominal respiration. Coughing was not a constant finding of the syndrome. At necropsy, macroscopic lesions included the overall appearance of pale animals, general lymphadenopathy, hepatic congestion, and consolidation of the lungs. Histopathologic findings were mainly proliferative pneumonia with a significant macrophage invasion, necrotic inflammatory cells in the alveoli and the airways, a marked proliferation of type II pneumocytes, and thickening of the alveolar septae. Fluorescent antibody examination of lungs of sick piglets did not demonstrate porcine parvovirus, transmissible gastroenteritis virus, or encephalomyocarditis virus. However, evidence of the presence of an influenza type A infection was demonstrated by indirect immunofluorescence (IIF) staining using monoclonal antibody directed to nucleocapsid protein (NP) of human type A influenza virus. The virus was isolated either by intra-allantoic inoculation of specific-pathogen-free embryonating hens' eggs or propagation in canine kidney (MDCK) cells in the presence of trypsin. By hemagglutination inhibition tests, no cross-reactivity was demonstrated with human influenza H1N1, H2N2, and H3N2 strains, and infected MDCK cells did not react by IIF with monoclonal antibodies to NP protein of type B influenza virus. The hemagglutination activity of plaque-purified isolates was only partly inhibited by hyperimmune serum produced to subtypes A/Wisconsin/76/H1N1 and A/New Jersey/76/H1N1 of swine influenza virus. Gnotobiotic piglets that were infected intranasally with egg-adapted isolates of this new antigenic variant of swine influenza virus developed the very same type of lesions observed in field cases.     

The second glutamic acid in the C-terminal CRD affects the carbohydrate-binding properties of recombinant galectins of Haemonchus contortus

The effects of the second glutamic acid (E) in the C-terminal CRDs on the hemagglutination and lactose-binding characteristics of the recombinant galectins of nematode Haemonchus contortus were observed using two isoforms of recombinant galectins as models, and the sugar-binding abilities of the N-terminal and C-terminal CRDs of the galectins were also compared. The second E in the CRD, WGNEER, of Hco-GAL-m was mutated to glycine acid (G) and resulted in a recombinant galectin (MG mutate) with a CRD of WGNEGR, identical to that of Hco-GAL-f. The G in Hco-GAL-f CRD, WGNEGR, was mutated to E and produced a recombinant galectin (FE mutate) equal to that of Hco-GAL-m. At the same time, the CRDs of the N-terminal (FNh,MNh) and C-terminal (FCh,MCh) of Hco-GAL-f, Hco-GAL-m were amplified by PCR. The abilities of carbohydrate binding and hemagglutination of the four galectins and the four CRDs were analysed, respectively, by alpha-lactose-agarose affinity chromatography and hemagglutination assay. The results showed that Hco-GAL-m and FE mutate bound effectively to alpha-lactose-agarose compared to Hco-GAL-f and MG mutate, which almost could not bind to the conjugate column. The hemagglutinating abilities of the Hco-GAL-m and FE mutate to human B type red blood cells were similar and were nearly two times higher than that of the Hco-GAL-f and MG mutate. The hemagglutinating ability of the MCh was five times to that of the MNh and FNh and almost two times to that of the FCh. The binding ability of the MCh and FCh were significantly reduced compared to that of the Hco-GAL-m and FE mutate, but still remained. As for the MNh and FNh, no elution peak was observed in the lactose-agarose affinity chromatography. These results suggested that the second amino acid E in the C-terminal CRD motif of H. contortus galectin was involved in carbohydrate binding and hemagglutination, and C-terminal CRDs had stronger carbohydrate ability than N-terminal CRDs.     

Receptor binding specificity and pathogenicity of Escherichia coli F165-positive strains isolated from piglets and calves and possessing pap related sequences.

Most of 82 F165-positive Escherichia coli isolated from calves and piglets with diarrhea or septicemia and possessing pap related sequences caused mannose-resistant, neuraminidase-resistant hemagglutination of human and bovine erythrocytes. Less than half of these isolates demonstrated binding specificity for the alpha-D-galactosyl-(1-4)-beta-D-galactopyranose or galactose-N-acetyl-alpha-(1-3) galactose-N-acetyl moieties recognized by P and F (or Prs) adhesins respectively. Binding specificity for the galactose-N-acetyl-alpha-(1-3) galactose-N-acetyl moiety was associated with isolates causing septicemia in newborn piglets.     

鸡新城疫病毒的简易纯化与电镜检测

用人Ｏ型红细胞吸附－释放病毒的方法纯化粪便中的鸡新城疫病毒（ＮＤＶ），然后再用电镜检查。结果表明，此法具有简便、快速、敏感等特点，可作为检测ＮＤＶ及其它具有血凝性病毒的常规方法推广应用。     

Pasteurella multocida (type D and A) and atrophic rhinitis of swine--hemagglutination, fimbriae and adhesion in vitro in the nasal mucosa of swine fetuses

79 strains of P. multocida were investigated, mostly isolated from porcine nasal cavities, and a mannose-resistant hemagglutination with guinea pig and human group 0, but not with porcine erythrocytes was found. Fimbriae as adhesins were demonstrated only on 2 strains. A correlation between capsular type, hemagglutination, fimbriation and toxigenicity on the examined P. multocida strains was not observed. Three strains were investigated for the adherence to the nasal mucosa of neonatal pigs; aggregates shown by scanning electron microscopy indicate colonization; a correlation of adherence with surface proteins and slime production of P. multocida is discussed.     

Complement-fixation and Hemagglutination Antigens from a Chlamydial (Ornithosis) Agent Grown in Cell Cultures

Methods are described for the preparation of complement-fixation (CF) and hemagglutination (HA) antigens from the Texas turkey ornithosis agent grown in McCoy cell culture monolayers. The particulate antigens prepared for this study were satisfactory for testing mammalian sera by direct CF tests and avian sera by indirect CF or modified direct CF tests. Comparison of titers were made on human, bovine and ovine sera using direct CF tests employing antigen prepared for this study, 6 BC yolk sac antigen, and a commercially available antigen.

The HA antigen agglutinated mouse erythrocytes, but it was not of value in hemagglutination inhibition tests because of “nonspecific” inhibitors in both mammalian and avian sera.

     

Diagnosis of histoplasmosis and blastomycosis by an antiglobulin hemagglutination test

An antiglobulin hemagglutination test was developed for detection of antibody directed to Histoplasma capsulatum and Blastomyces dermatitidis. The substances responsible for spontaneous agglutination of erythrocytes were removed from histoplasmin and blastomycin by vacuum dialysis, and partial purification of the antigens by gel filtration chromatography on Sephadex G-150 allowed removal of additional nonantigenic material which competed with the antigens for binding on the erythrocyte surface. The test was sensitive enough to detect antibodies in sera which were negative by complement fixation, immunodiffusion, or both, but it failed to discriminate reliably between antibody directed to H capsulatum and antibody directed to B dermatitidis. Erythrocytes sensitized with partially purified blastomycin produced some false-positive reactions with normal canine sera; this was corrected by diluting the antigen before sensitization of the erythrocytes.     

Hemagglutinating activity associated with bovine herpesvirus type 1

Using C57BL/HPB mouse erythrocytes, hemagglutination has been observed with the Los Angeles and Colorado-1 strains of bovine herpesvirus type 1 and with 12 other Canadian field isolates as well. The specificity of the hemagglutination observed with the viral strains has been confirmed by a hemagglutination-inhibition assay.     

鸭源新城疫病毒的分离鉴定

从病死肉鸭肝脏中分离到2株病毒(ZH1、ZH2),均能够凝集鸡、肉鸭、绵羊、山羊、猪、人、兔、牛等的红细胞,且这种血凝性可被NDV标准阳性血清所抑制.参照NDV毒力判定标准及其方法对分离毒株ZH1、ZH2进行了鸡胚最小致死量平均死亡时间(MDT)、鸡胚半数感染量(EID50)以及1日龄鸡脑内接种致病指数(ICPI)测定,结果ZH1、ZH2株的MDT为52 h和44 h,EID50为106.4/0.1mL和108.64/0.1mL,ICPI为1.93和1.975.表明这2株分离病毒均为NDV强毒株.