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Effects of various substances on the binding of keratin monomers to S. maltophilia DHHJ cells for the induction of keratinase production.
Xue, Kai; Song, XiaoXiao; Zhang, Wei; Zhang, YunLong; Cao, ZhangJun; Zhang, XingQun; Zhang, ZhongGe.
Affiliation
  • Xue K; College of Biological Science and Medical Engineering, Donghua University, Shanghai, 201620, China.
  • Song X; College of Biological Science and Medical Engineering, Donghua University, Shanghai, 201620, China.
  • Zhang W; College of Biological Science and Medical Engineering, Donghua University, Shanghai, 201620, China.
  • Zhang Y; College of Biological Science and Medical Engineering, Donghua University, Shanghai, 201620, China.
  • Cao Z; College of Biological Science and Medical Engineering, Donghua University, Shanghai, 201620, China. zhjcao@dhu.edu.cn.
  • Zhang X; Key Laboratory of Science & Technology of Eco-Textile, Ministry of Education, Donghua University, Shanghai, 201620, China. zhjcao@dhu.edu.cn.
  • Zhang Z; National Engineering Research Center for Dyeing and Finishing of Textiles, Donghua University, Shanghai, 201620, People's Republic of China. zhjcao@dhu.edu.cn.
Article in En | MEDLINE | ID: mdl-38896367
ABSTRACT
Biodegradation effectiveness of S. maltophilia DHHJ is determined by its ability to attach to the hydrolyzed feather keratin monomers. This binding capacity can be influenced by many components in the culture medium. Keratin monomers from feathers or those produced by gene overexpression can induce keratinase production in S. maltophilia DHHJ, and several proteases lack the ability to degrade keratin fragments and cysteines. In this study, we co-incubated FITC-labelled keratin monomers with S. maltophilia DHHJ cells in the presence of BSA, DNA, ATP, and several metal ions, and measured fluorescence values and keratinase activity. BSA was found to compete with keratins for cell binding sites, resulting in less keratinase production. DNA did not interfere with cellular binding to keratins revealing unchanged keratinase level. ATP, along with metal ions, enhanced the cellular binding capacity to keratins and increased the production of keratinase by S. maltophilia DHHJ. Fragments of keratin monomers degraded by proteases reduced the ability of cells to bind to keratin and affected enzyme production. Cysteine, a characteristic amino acid of feather keratin, did not have an effect on cellular binding to keratin monomer or on keratinase production. This study will facilitate the tweaking of catalytic parameters to improve feather biodegradation by S. maltophilia DHHJ.
Key words

Full text: 1 Collection: 01-internacional Database: MEDLINE Language: En Journal: Appl Biochem Biotechnol Year: 2024 Document type: Article Affiliation country: China Country of publication: United States

Full text: 1 Collection: 01-internacional Database: MEDLINE Language: En Journal: Appl Biochem Biotechnol Year: 2024 Document type: Article Affiliation country: China Country of publication: United States