ZHAO Xiao Tao; FENG Jiang Bin; LI Yu Wen; LUO Qun; YANG Xin Chun; LU Xue; CHEN De Qing; LIU Qing Jie

doi:10.3967/0895-3988.2012.05.006

Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation

ZHAO Xiao Tao, FENG Jiang Bin, LI Yu Wen, LUO Qun, YANG Xin Chun, LU Xue, CHEN De Qing, LIU Qing Jie

文章导航 > Biomedical and Environmental Sciences > 2012 > 25(5): 533-541

ZHAO Xiao Tao, FENG Jiang Bin, LI Yu Wen, LUO Qun, YANG Xin Chun, LU Xue, CHEN De Qing, LIU Qing Jie. Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation[J]. Biomedical and Environmental Sciences, 2012, 25(5): 533-541. doi: 10.3967/0895-3988.2012.05.006

Citation:

ZHAO Xiao Tao, FENG Jiang Bin, LI Yu Wen, LUO Qun, YANG Xin Chun, LU Xue, CHEN De Qing, LIU Qing Jie. Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation[J]. Biomedical and Environmental Sciences, 2012, 25(5): 533-541. doi: 10.3967/0895-3988.2012.05.006

doi: 10.3967/0895-3988.2012.05.006

基金项目: the National Natural Science Foundation of China(30570551%30870749)%the Beijing Natural Science Foundation(7053073)

Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation

Department of Cardiology,Beijing Chao-Yang Hospital,Capital Medical University,Beijing 100020,China
Key Laboratory of Radiological Protection and Nuclear Emergency,National Institute for Radiological Protection,Chinese Center for Disease Control and Prevention,Beijing 100088,China
Department of Transfusion,Chinese PLA General Hospital,Beijing 100853,China

Funds: the National Natural Science Foundation of China(30570551%30870749)%the Beijing Natural Science Foundation(7053073)

摘要: Objective We identify ionizing radiation‐induced mitochondrial DNA (mtDNA) deletions in human lymphocytes and their distribution in normal populations. Methods Long‐range polymerase chain reactions (PCR) using two pairs of primers specific for the human mitochondrial genome were used to analyze the lymphoblastoid cell line following exposure to 10 Gy 60Co γ‐rays. Limited‐condition PCR, cloning and sequencing techniques were applied to verify the mtDNA deletions detected with long‐range PCR. Human peripheral blood samples were irradiated with 0, 2 and 6 Gy 60Co γ‐rays, and real‐time PCR analysis was performed to validate the mtDNA deletions. In order to know the distribution of mtDNA deletions in normal population, 222 healthy Chinese adults were also investigated. Results Two mtDNA deletions, a 7455‐bp deletion (nt475‐nt7929 in heavy strand) and a 9225‐bp deletion (nt7714 ‐nt369 in heavy strand), occurring between two 8‐bp direct repeats, were identified in lymphoblastoid cells using long‐range PCR, limited‐condition PCR and sequencing. These results were also observed for 60Co γ‐rays irradiated human peripheral blood cells. Conclusion Two novel mtDNA deletions, a 7455‐bp deletion and a 9225‐bp deletion, were induced by ionizing radiation. The rate of the mtDNA deletions within a normal population was related to the donors’ age, but was independent of gender.
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Abstract: Objective We identify ionizing radiation‐induced mitochondrial DNA (mtDNA) deletions in human lymphocytes and their distribution in normal populations. Methods Long‐range polymerase chain reactions (PCR) using two pairs of primers specific for the human mitochondrial genome were used to analyze the lymphoblastoid cell line following exposure to 10 Gy 60Co γ‐rays. Limited‐condition PCR, cloning and sequencing techniques were applied to verify the mtDNA deletions detected with long‐range PCR. Human peripheral blood samples were irradiated with 0, 2 and 6 Gy 60Co γ‐rays, and real‐time PCR analysis was performed to validate the mtDNA deletions. In order to know the distribution of mtDNA deletions in normal population, 222 healthy Chinese adults were also investigated. Results Two mtDNA deletions, a 7455‐bp deletion (nt475‐nt7929 in heavy strand) and a 9225‐bp deletion (nt7714 ‐nt369 in heavy strand), occurring between two 8‐bp direct repeats, were identified in lymphoblastoid cells using long‐range PCR, limited‐condition PCR and sequencing. These results were also observed for 60Co γ‐rays irradiated human peripheral blood cells. Conclusion Two novel mtDNA deletions, a 7455‐bp deletion and a 9225‐bp deletion, were induced by ionizing radiation. The rate of the mtDNA deletions within a normal population was related to the donors’ age, but was independent of gender.
- Mitochondrial DNA deletion /
- Ionizing radiation /
- Lymphocytes /
- Chinese adults

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Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation

doi: 10.3967/0895-3988.2012.05.006

基金项目: the National Natural Science Foundation of China(30570551%30870749)%the Beijing Natural Science Foundation(7053073)

刊出日期: 2012-10-20

关键词:

Mitochondrial DNA deletion /

Ionizing radiation /

Lymphocytes /

Chinese adults

摘要: Objective We identify ionizing radiation‐induced mitochondrial DNA (mtDNA) deletions in human lymphocytes and their distribution in normal populations. Methods Long‐range polymerase chain reactions (PCR) using two pairs of primers specific for the human mitochondrial genome were used to analyze the lymphoblastoid cell line following exposure to 10 Gy 60Co γ‐rays. Limited‐condition PCR, cloning and sequencing techniques were applied to verify the mtDNA deletions detected with long‐range PCR. Human peripheral blood samples were irradiated with 0, 2 and 6 Gy 60Co γ‐rays, and real‐time PCR analysis was performed to validate the mtDNA deletions. In order to know the distribution of mtDNA deletions in normal population, 222 healthy Chinese adults were also investigated. Results Two mtDNA deletions, a 7455‐bp deletion (nt475‐nt7929 in heavy strand) and a 9225‐bp deletion (nt7714 ‐nt369 in heavy strand), occurring between two 8‐bp direct repeats, were identified in lymphoblastoid cells using long‐range PCR, limited‐condition PCR and sequencing. These results were also observed for 60Co γ‐rays irradiated human peripheral blood cells. Conclusion Two novel mtDNA deletions, a 7455‐bp deletion and a 9225‐bp deletion, were induced by ionizing radiation. The rate of the mtDNA deletions within a normal population was related to the donors’ age, but was independent of gender.

English Abstract

Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation

Department of Cardiology,Beijing Chao-Yang Hospital,Capital Medical University,Beijing 100020,China

Key Laboratory of Radiological Protection and Nuclear Emergency,National Institute for Radiological Protection,Chinese Center for Disease Control and Prevention,Beijing 100088,China

Department of Transfusion,Chinese PLA General Hospital,Beijing 100853,China

Funds: the National Natural Science Foundation of China(30570551%30870749)%the Beijing Natural Science Foundation(7053073)

Publish Date: 2012-10-20

Keywords:

Abstract: Objective We identify ionizing radiation‐induced mitochondrial DNA (mtDNA) deletions in human lymphocytes and their distribution in normal populations. Methods Long‐range polymerase chain reactions (PCR) using two pairs of primers specific for the human mitochondrial genome were used to analyze the lymphoblastoid cell line following exposure to 10 Gy 60Co γ‐rays. Limited‐condition PCR, cloning and sequencing techniques were applied to verify the mtDNA deletions detected with long‐range PCR. Human peripheral blood samples were irradiated with 0, 2 and 6 Gy 60Co γ‐rays, and real‐time PCR analysis was performed to validate the mtDNA deletions. In order to know the distribution of mtDNA deletions in normal population, 222 healthy Chinese adults were also investigated. Results Two mtDNA deletions, a 7455‐bp deletion (nt475‐nt7929 in heavy strand) and a 9225‐bp deletion (nt7714 ‐nt369 in heavy strand), occurring between two 8‐bp direct repeats, were identified in lymphoblastoid cells using long‐range PCR, limited‐condition PCR and sequencing. These results were also observed for 60Co γ‐rays irradiated human peripheral blood cells. Conclusion Two novel mtDNA deletions, a 7455‐bp deletion and a 9225‐bp deletion, were induced by ionizing radiation. The rate of the mtDNA deletions within a normal population was related to the donors’ age, but was independent of gender.

Citation:

ZHAO Xiao Tao, FENG Jiang Bin, LI Yu Wen, LUO Qun, YANG Xin Chun, LU Xue, CHEN De Qing, LIU Qing Jie. Identification of Two Novel Mitochondrial DNA Deletions Induced by Ionizing Radiation[J]. Biomedical and Environmental Sciences, 2012, 25(5): 533-541. doi: 10.3967/0895-3988.2012.05.006