Sapelovirus A (SV-A) is a positive-sense single-stranded RNA virus which is associated with acute diarrhea, pneumonia and reproductive disorders. The virus capsid is composed of four proteins, and the functions of the structural proteins are unclear. In this study, we expressed SV-A structural protein VP1 and studied its antigenicity and immunogenicity. SDS-PAGE analysis revealed that the target gene was expressed at high levels at 0.6 mM concentration of IPTG for 24 h. The mouse polyclonal antibody against SV-A VP1 protein was produced and reached a high antiserum titer (1: 2,048,000). Immunized mice sera with the recombinant SV-A VP1 protein showed specific recognition of purified VP1 protein by western blot assay and could recognize native SV-A VP1 protein in PK-15 cells infected with SV-A by indirect immunofluorescence assay. The successfully purified recombinant protein was able to preserve its antigenic determinants and the generated mouse anti-SV-A VP1 antibodies could recognize native SV-A, which may have the potential to be used to detect SV-A infection in pigs.
Osteocalcin is a major non-collagenous component of the bone extracellular matrix and is considered to be an indicative factor of osteoblast differentiation. In the present study, we detected osteocalcin expression in different antler areas and growth phases by immunohisto- chemistry. Osteocalcin was highly expressed in all areas during the mineralization period and in mesenchymal cell and chondrocyte areas during the rapid growth period. The nucleotide sequence of the osteocalcin gene in sika deer antler was determined. The open reading frame was 303 bp encoding a protein of 100 amino acids. The estimated molecular mass of osteocalcin was 10.38 kDa and the theoretical isoelectric point was 5.37. The osteocalcin gene with a 6× His-tag at the C-terminus was cloned into the pGEX-4T1 vector and expressed in Escherichia coli under optimal conditions. The recombinant soluble protein fused with GST was purified with Ni-NTA resin. The purified osteocalcin protein exhibited a significant increase in HA adhesion and promoted antler chondrocyte proliferation. Osteocalcin is an important factor in regulating the rapid growth and differentiation of deer antlers.
This article presents the effects of the application of the passive method of flue gas purification from mercury compounds emitted during combustion. The research was carried out on a fluidized bed installation using coal. The dry method of acid gas pollutants reduction was applied during the combustion with the use of 9 modified sodium sorbents. They were fed into a gas jet of 573 K in two molar ratios (sodium contained in the sorbent to the sulphur contained in the fuel). The mercury emission level into the atmosphere was determined based on the mercury content in the solid substrates of the combustion process (in the fuel and the sorbent) and the solid products (fly ash and bottom waste). The combustion process was accompanied by mercury emission 14.7 μgHg/m3. During the removal of acid pollutants from fumes, a decrease in mercury concentration was achieved. The degree of the mercury reduction depended on the type the sorbent used, the manner of modification and the molar ratio in which they were fed into the installation (2 Na/S = 0.5; 2.1). Each time, the more the sorbent was fed into the installation, the bigger the reduction of the mercury emission level. Among the unmodified sorbents, the lowest emission level was achieved for the raw bicarbonate – 3.7 μgHg/m3. For baking soda it was 9.7 μgHg/m3. The application of mechanically modified compounds based on baking soda resulted in the reduction of the Hg emission in fumes up to 2.5–2.6 μgHg/m3. The determined mercury concentration levels in the gases during the purification of the fumes were compared with the accepted Hg emissions contained in the BAT conclusions for large combustion plants. As for all of the existing and newly built plants with a heat capacity below 300 MW, satisfactory effects would be achieved by the use of mechanically modified sorbents in the molar concentration of 2 Na/S = 2.1.
Biological regeneration of water and organic sorbents used in the absorption of hydrophilic and hydrophobic pollutants, respectively, was studied. In both cases biodegradation takes place in a membrane bioreactor. In the case of organic sorbents regeneration of the biodegradation process is integrated with the extraction of a given pollutant to water phase. In experiments carried out in this work, the proposed systems were tested using a strain of Pseudomonas fluorescens. For hydrophilic compounds experiments were performed using alcohols (1-butanol and 2-propanol) as model substrates. Applying the mathematical model of a membrane bioreactor elaborated previously, the values of pollutant concentration were determined and positively verified in the experiments. This system of water sorbent regeneration is fully satisfying. The process of biodegradation integrated with extraction was analysed on the basis of model compounds such as benzene and toluene. The study confirmed a possibility of organic sorbent (silicone oil) regeneration. However, due to a very high partition coefficient of benzene or toluene between the organic and aqueous phases, the process could be considered only for the case of their high concentrations in the gas directed to absorption.