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Optimization of Fungal Dextranase Production and Its Antibiofilm Activity Encapsulation and Stability in Toothpaste

机译:真菌葡聚糖酶生产的优化及其抗牙膏封装和稳定性

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摘要

Dextranase catalyzes the degradation of the substrate dextran, which is a component of plaque biofilm. This enzyme is involved in antiplaque accumulation, which can prevent dental caries. The activity of crude dextranase from Penicillium roquefortii TISTR 3511 was assessed, and the maximum value (7.61 unit/g) was obtained at 37 °C and pH 6. The Plackett–Burman design was used to obtain significant factors for enhancing fungal dextranase production, and three influencing factors were found: Dextran, yeast extract concentration and inoculum age. Subsequently, the significant factors were optimized with the Box–Behnken design, and the most suitable condition for dextranase activity at 30.24 unit/g was achieved with 80 g/L dextran, 30 g/L yeast extract and five day- old inoculum. The use of 0.85% alginate beads for encapsulation exhibited maximum dextranase activity at 25.18 unit/g beads, and this activity was stable in toothpaste for three months of testing. This study explored the potential production of fungal dextranase under optimal conditions and its encapsulation using alginate for the possibility of applying encapsulated dextranase as an additive in toothpaste products for preventing dental caries.
机译:葡聚糖酶催化基材葡聚糖的降解,这是斑块生物膜的组分。该酶参与抗薄层积累,可以防止龋齿。评估来自roquefortii TISTR 3511的粗葡聚糖酶的活性,并在37℃和pH 6中获得最大值(7.61单位/ g).PRAKET-BURMAN设计用于获得增强真菌葡聚糖酶生产的重要因素,发现了三种影响因素:葡聚糖,酵母提取物浓度和接种症。随后,通过箱Behnken设计进行了显着因素,并使用80g / L葡聚糖,30g / L酵母提取物和五天古老的接种物,实现了30.24单元/ g的最合适的葡聚糖酶活性条件。使用0.85%的藻酸盐珠粒用于包封在25.18单位/克珠粒上表现出最大的葡聚糖酶活性,并且该活性在牙膏中稳定为3个月的测试。本研究探讨了在最佳条件下潜在生产的潜在生产及其使用藻酸盐的封装,以便将包封的葡聚糖酶应用于牙膏产品中的添加剂,以防止龋齿。

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