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At present, there is no effective experimental method for detecting whether the suid herpesvirus 1 (SHV-1) detected in pigs is infectious. Although the technique of quantitative polymerase chain reaction (qPCR) has significantly improved the detection rate and accuracy of the disease, it does not differentiate between infective and non-infective status of the virus. Propidium monoazide (PMA) is a dye that can be combined with DNA molecules. The decomposition of PMA produces an azene compound covalently crosslinked with DNA molecules, thereby inhibiting PCR amplification of DNA. In this study, the combination of PMA and qPCR was used to determine the infectivity of SHV-1. We optimized the method from the selection of primers, the working concentration of PMA, and the method of inactivation using UV or heat inactivation. We found that when specific primer 1 was used and a PMA working concentration was 50-100 µM, heat inactivation was able to distinguish whether SHV-1 was infectious or not. We also showed that UV prevented the virus from replicating, it did not destroy the capsid of the virus, and therefore, PMA cannot enter the virus and bind to the nucleic acid of the virus. Consequently, there is no way to identify the infectivity of the virus using UV inactivation. The study showed that the method was stable and the detection rate reached 96%. In conclusion, this method exhibited strong specificity and high sensitivity and can identify the infectivity of SHV-1. This method has practical significance for clinical virus isolation and the effects of disinfection of farms.
RESUMO
Reverse transcription-quantitative polymerase chain reaction (RT-qPCR) allows sensitive detection of viral particles and viruses in epidemic samples but it cannot discriminate noninfectious viruses from infectious ones. Propidium monoazide (PMA) coupled with quantitative polymerase chain reaction (qPCR) was assessed to detect infectious viruses. Currently, there is no established test method to detect the infection of the porcine epidemic diarrhea virus (PEDV). In this study, propidium monoazide coupled with qPCR detects infectivity of PEDV. We optimized the method from the selection of primers, the working concentration of PMA, and the inactivation method using heat or ultraviolet (UV). The viruses which were treated with PMA before qPCR were inactivated using heat or UV. However, the addition of PMA alone did not affect the detection of live viruses, which indicates that a viral capsid break may be essential for PMA to bind to the genome. A repetition of the method on naked PEDV RNA suggests that it can be used to detect potentially infectious PEDV. The results indicated that an optimal plan of PMA could be extremely useful for evaluating infectious and noninfectious viruses.
RESUMO
Porcine circovirus type 2 (PCV2) is one of the smallest known animal viruses and is the main pathogen of PCV-associated diseases (PCVAD). Epidemiological surveillance results have shown that the PCV2 infection rate is on the rise in China, thus, PCV2 disease prevention and control has become a huge challenge for the Chinese swine industry. We collected clinical samples from multiple different provinces in China from 2018 to 2020 and found that the positive rate of PCV2 was 53% (3619/6872), identity between the cloned 62 ORF2 genes was 84.4-100% and identity between the cloned 62 ORF2 sequences and reference sequence was 72.9-99.8%. Genetic evolution analysis found that PCV2d accounted for 79% (49/62 samples), PCV2a for 12.9% (8/62 samples), PCV2b for 8% (5/62 samples), and PCV2c and PCV2e genotypes were not found. However, most commercial PCV2 subunit vaccines are based on the PCV2a genotype, and there are very few vaccines based on PCV2b or PCV2d. Therefore, the homologous and heterologous protection ability of PCV2b and PCV2d Cap proteins based on the baculovirus against the PCV2b and PCV2d infections was evaluated, which is expected to design and develop excellent PCV2 protein vaccine candidates. This study found that both PCV2b and PCV2d Cap proteins can increase the level of humoral immunity and cellular immune response in mice. Importantly, both PCV2b and PCV2d cap proteins can provide homologous and heterologous protection against the PCV2b and PCV2d viruses. Overall, this study provides a reference for the prevention and control of PCVAD in mainland China and the development of PCV2 vaccines.
RESUMO
The random disposal and incineration of agricultural residues cause resources waste and environmental pollution. The potential of waste biomass for the production of alternative liquid fuels is increasing and the bioconversion of lignocellulose to fermentable monomeric sugars is essential for second-generation biofuel production. Here, natural and pretreated switch grass or rice straw were fermented by both Trichoderma asperellum T-1 and Trichoderma reesei QM6a, with the fermentation results highlighted the potential of T. asperellum T-1 in the degradation of natural waste lignocellulosic materials. In fermenting different substrates, the filter paper activity, ß-glucosidase activity, xylanase activity and carboxymethyl cellulase activity of T-1 can respectively reach 1.88, 8.00, 7.15 and 20.52 times that of QM6a. Although acid pretreatment could improve the enzyme activities of both T-1 and QM6a, its effect on T-1 was much smaller than that on QM6a. Moreover, strain T-1 fermented the natural rice straw better than the pretreated rice straw. Therefore, T-1 is considered to be more suitable for the degradation of natural biomass, especially for the degradation of rice straw. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and scanning electron microscopy (SEM) showed that the cellulase series secreted by T. asperellum T-1 was more abundant, and its substrate deconstruction ability was stronger than T. reesei QM6a. All these results suggest the potential of T. asperellum T-1 in the degradation of natural waste lignocellulosic material, with practical benefits in terms of cost and pollution reduction.
RESUMO
BACKGROUND: Agricultural waste is as an alternative low-cost carbon source or beneficial additives which catch most people's eyes. In addition, methanol and sweet potato vine hydrolysate (SVH) have been reported as the efficient enhancers of fermentation according to some reports. The objective of the present study was to confirm SVH as an efficient additive in CA production and explore the synergistic effects of methanol and SVH in fermentation reactions. RESULTS: The optimal fermentation conditions resulted in a maximum citric acid concentration of 3.729 g/L. The final citric acid concentration under the optimized conditions was increased by 3.6-fold over the original conditions, 0.49-fold over the optimized conditions without methanol, and 1.8-fold over the optimized conditions in the absence of SVH. Kinetic analysis showed that Qp, Yp/s, and Yx/s in the optimized systems were significantly improved compared with those obtained in the absence of methanol or SVH. Further, scanning electron microscopy (SEM) revealed that methanol stress promoted the formation of conidiophores, while SVH could neutralize the effect and prolong Aspergillus niger vegetative growth. Cell viability analysis also showed that SVH might eliminate the harmful effects of methanol and enhance cell membrane integrity. CONCLUSIONS: SVH was a superior additive for organic acid fermentation, and the combination of methanol and SVH displayed a significant synergistic effect. The research provides a preliminary theoretical basis for SVH practical application in the fermentation industry.
RESUMO
The bacterial expansin, BsEXLX1, has been studied as a model to understand the synergistic effect of expansins on lignocellulose degradation and the structure-function relationships of expansins. However, the specific mechanism is still poorly understood. In this study, the binding, synergistic and structural characteristics of BsEXLX1 for loosening the main components of lignocellulose: lignin, xylan, and cellulose, were further characterized. Results showed that BsEXLX1 preferentially binds to xylan over lignin or cellulose under various conditions. The binding of BsEXLX1 to all substrates increased linearly with the initial concentration of BsEXLX1. But the changing rate of binding (i.e., slope of the line; k value) varied with the incubation temperature. Interestingly, the binding of BsEXLX1 to substrates did not saturate. Mutating residue-125, 126 or 171 indicated their importance for binding, but they were less important for binding to xylan. Through binding assays and homologous modeling, it was concluded that residue-125 and 171 play more important roles in the structural maintenance of BsEXLX1. By comparing the synergistic activity of BsEXLX1 or its mutants, it was found that synergistic activity is not correlated with specific binding. All these results can lead deeper understand about the mechanism of wall loosening by expansins, and further promote the application of expansins in lignocellulose degradation.