Comparative genomic sequencing to characterize genome, typing, and drug resistance.
Yue Jiang, Hailong Kang, Haiwei Dou, Dongxing Guo, Qing Yuan, Lili Dong, Zhenglin Du, Wenming Zhao, Deli Xin
Author Information
Yue Jiang: Pediatric Department, Beijing Chao-Yang Hospital, Capital Medical University, Beijing, China. ORCID
Hailong Kang: National Genomics Data Center and CAS Key Laboratory of Genome Sciences and Information, Beijing Institute of Genomics, Chinese Academy of Sciences and China National Center for Bioinformation, Beijing, China. ORCID
Haiwei Dou: Tropical Medicine Research Institute, Beijing Friendship Hospital, Capital Medical University, Beijing, China.
Dongxing Guo: Tropical Medicine Research Institute, Beijing Friendship Hospital, Capital Medical University, Beijing, China.
Qing Yuan: Tropical Medicine Research Institute, Beijing Friendship Hospital, Capital Medical University, Beijing, China.
Lili Dong: National Genomics Data Center and CAS Key Laboratory of Genome Sciences and Information, Beijing Institute of Genomics, Chinese Academy of Sciences and China National Center for Bioinformation, Beijing, China.
Zhenglin Du: National Genomics Data Center and CAS Key Laboratory of Genome Sciences and Information, Beijing Institute of Genomics, Chinese Academy of Sciences and China National Center for Bioinformation, Beijing, China.
Wenming Zhao: National Genomics Data Center and CAS Key Laboratory of Genome Sciences and Information, Beijing Institute of Genomics, Chinese Academy of Sciences and China National Center for Bioinformation, Beijing, China. ORCID
Deli Xin: Tropical Medicine Research Institute, Beijing Friendship Hospital, Capital Medical University, Beijing, China. ORCID
To analyze the characteristics of as well as macrolide antibiotic resistance through whole-genome sequencing and comparative genomics. Thirteen clinical strains isolated from 2003 to 2019 were selected, 10 of which were resistant to erythromycin (MIC >64 ��g/mL), including 8 P1-type I and 2 P1-type II. Three were sensitive (<1 ��g/mL) and P1-type II. One resistant strain had an A���G point mutation at position 2064 in region V of the 23S rRNA, the others had it at position 2063, while the three sensitive strains had no mutation here. Genome assembly and comparative genome analysis revealed a high level of genome consistency within the P1 type, and the primary differences in genome sequences concentrated in the region encoding the P1 protein. In P1-type II strains, three specific gene mutations were identified: C162A and A430G in L4 gene and T1112G mutation in the CARDS gene. Clinical information showed seven cases were diagnosed with severe pneumonia, all of which were infected with drug-resistant strains. Notably, BS610A4 and CYM219A1 exhibited a gene multi-copy phenomenon and shared a conserved functional domain with the DUF31 protein family. Clinically, the patients had severe refractory pneumonia, with pleural effusion, necessitating treatment with glucocorticoids and bronchoalveolar lavage. The primary variations between strains occur among different P1-types, while there is a high level of genomic consistency within P1-types. Three mutation loci associated with specific types were identified, and no specific genetic alterations directly related to clinical presentation were observed.IMPORTANCE is an important pathogen of community-acquired pneumonia, and macrolide resistance brings difficulties to clinical treatment. We analyzed the characteristics of as well as macrolide antibiotic resistance through whole-genome sequencing and comparative genomics. The work addressed primary variations between strains that occur among different P1-types, while there is a high level of genomic consistency within P1-types. In P1-type II strains, three specific gene mutations were identified: C162A and A430G in L4 gene and T1112G mutation in the CARDS gene. All the strains isolated from severe pneumonia cases were drug-resistant, two of which exhibited a gene multi-copy phenomenon, sharing a conserved functional domain with the DUF31 protein family. Three mutation loci associated with specific types were identified, and no specific genetic alterations directly related to clinical presentation were observed.
