Screening Key Sites of Class 2 Integron Integrase that Impact Recombination Efficiency

被引:0
|
作者
Wang, Xiaotong [1 ,2 ]
Dai, Yueru [1 ]
Kong, Nana [1 ]
Cao, Mei [1 ]
Zhang, Long [1 ]
Wei, Quhao [1 ,3 ,4 ]
机构
[1] Anhui Univ Sci & Technol, Affiliated Fengxian Hosp, Dept Lab Med, 6600 Nanfeng Rd, Shanghai 201499, Peoples R China
[2] Shanghai Jiao Tong Univ, Songjiang Hosp, Sch Med, Clin Lab, 748 Middle Zhongshan Rd, Shanghai 201602, Peoples R China
[3] Southern Med Univ, Affiliated Fengxian Hosp, Dept Lab Med, 6600 Nanfeng Rd, Shanghai 201499, Peoples R China
[4] Shanghai Univ Med & Hlth Sci, Affiliated Peoples Hosp South Campus 6, Dept Lab Med, 6600 Nanfeng Rd, Shanghai 201499, Peoples R China
基金
中国国家自然科学基金;
关键词
ANTIBIOTIC-RESISTANCE; BACTERIAL-RESISTANCE; 59-BASE ELEMENT; CASSETTES; GENES; INTI1;
D O I
10.1007/s00284-024-03674-0
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
By capturing and expressing exogenous resistance gene cassettes through site-specific recombination, integrons play important roles in the horizontal transfer of antimicrobial resistant genes among bacteria. The characteristics of integron integrase make it to be a potential gene editing tool enzyme. In this study, a random mutation library using error-prone PCR was constructed, and amino acid residues mutants that impact on attI2 x attC or attC x attC recombination efficiency were screened and analyzed. Thirteen amino acid mutations were identified to be critical impacted on site-specific recombination of IntI2, including the predicted catalyzed site Y301. Nine of 13 mutated amino acid residues that have critically impacted on IntI2 activity were relative concentrated and near the predicted catalyzed site Y301 in the predicted three-dimensional structure indicated the importance of this area in maintain the activity of IntI2. No mutant with obviously increased recombination activity (more than four-fold as high as that of wild IntI2) was found in library screening, except P95S, R100K slightly increased (within two-fold) the excision activity of IntI2, and S243T slightly increased (within two-fold) both excision and integration activity of IntI2. These findings will provide clues for further specific modification of integron integrase to be a tool enzyme as well as establishing a new gene editing system and applied practically.
引用
收藏
页数:11
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