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Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome

DNA ligases I and II were separated by hydroxylapatite (HA) column chromatography in cell‐free extracts of lymphoblastoid cell lines (LCLs) derived from two unrelated patients with Bloom's syndrome (BS) and two healthy individuals. The specific activity of ligase I from the crude extract was co...

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Autores principales: Kurihara, Takayuki, Teraoka, Hirobumi, Inoue, Masao, Takebe, Hiraku, Kouichi, Kouichi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Blackwell Publishing Ltd 1991
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5918217/
https://www.ncbi.nlm.nih.gov/pubmed/1900268
http://dx.doi.org/10.1111/j.1349-7006.1991.tb01745.x
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author Kurihara, Takayuki
Teraoka, Hirobumi
Inoue, Masao
Takebe, Hiraku
Kouichi, Kouichi
author_facet Kurihara, Takayuki
Teraoka, Hirobumi
Inoue, Masao
Takebe, Hiraku
Kouichi, Kouichi
author_sort Kurihara, Takayuki
collection PubMed
description DNA ligases I and II were separated by hydroxylapatite (HA) column chromatography in cell‐free extracts of lymphoblastoid cell lines (LCLs) derived from two unrelated patients with Bloom's syndrome (BS) and two healthy individuals. The specific activity of ligase I from the crude extract was consistently lower in GM3403, a BS LCL from an Ashkenazi Jewish patient, than in normal control LCLs. By contrast, the level of ligase I activity in BSL‐2KA, another BS LCL derived from a Japanese patient, was equivalent to those in normal LCLs, although GM3403 and BSL‐2KA shared the feature of exceedingly high frequency of spontaneous sister‐chromatid exchange. The levels of total ligase activity in crude extracts without the separation into the two forms, however, were approximately two‐fold higher for the two BS LCLs than for the normal LCLs. Partial purification by chromatography on a DEAE‐cellulose 23 column and a phosphocellulose column did not affect the superiority of the two BS LCLs over the normal LCLs in the specific activity of the total ligases. Nonetheless, subsequent application to an HA column again resulted in much less elevation of the specific activity of ligase I for GM3403 than for BSL‐2KA and control LCLs. The levels of ligase II activity, accounting for 4‐13% of total ligase activity, were similar among the LCLs examined. Irrespective of the extent of purification, essentially no difference in the heat lability of DNA ligase I was detected among the four LCLs. These findings suggest that there may exist among BS LCLs at least two types of subtle abnormality of DNA ligase I itself and/or a putative substance modulating the enzyme function.
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spelling pubmed-59182172018-05-11 Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome Kurihara, Takayuki Teraoka, Hirobumi Inoue, Masao Takebe, Hiraku Kouichi, Kouichi Jpn J Cancer Res Article DNA ligases I and II were separated by hydroxylapatite (HA) column chromatography in cell‐free extracts of lymphoblastoid cell lines (LCLs) derived from two unrelated patients with Bloom's syndrome (BS) and two healthy individuals. The specific activity of ligase I from the crude extract was consistently lower in GM3403, a BS LCL from an Ashkenazi Jewish patient, than in normal control LCLs. By contrast, the level of ligase I activity in BSL‐2KA, another BS LCL derived from a Japanese patient, was equivalent to those in normal LCLs, although GM3403 and BSL‐2KA shared the feature of exceedingly high frequency of spontaneous sister‐chromatid exchange. The levels of total ligase activity in crude extracts without the separation into the two forms, however, were approximately two‐fold higher for the two BS LCLs than for the normal LCLs. Partial purification by chromatography on a DEAE‐cellulose 23 column and a phosphocellulose column did not affect the superiority of the two BS LCLs over the normal LCLs in the specific activity of the total ligases. Nonetheless, subsequent application to an HA column again resulted in much less elevation of the specific activity of ligase I for GM3403 than for BSL‐2KA and control LCLs. The levels of ligase II activity, accounting for 4‐13% of total ligase activity, were similar among the LCLs examined. Irrespective of the extent of purification, essentially no difference in the heat lability of DNA ligase I was detected among the four LCLs. These findings suggest that there may exist among BS LCLs at least two types of subtle abnormality of DNA ligase I itself and/or a putative substance modulating the enzyme function. Blackwell Publishing Ltd 1991-01 /pmc/articles/PMC5918217/ /pubmed/1900268 http://dx.doi.org/10.1111/j.1349-7006.1991.tb01745.x Text en
spellingShingle Article
Kurihara, Takayuki
Teraoka, Hirobumi
Inoue, Masao
Takebe, Hiraku
Kouichi, Kouichi
Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title_full Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title_fullStr Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title_full_unstemmed Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title_short Two Types of DNA Ligase I Activity in Lymphoblastoid Cells from Patients with Bloom's Syndrome
title_sort two types of dna ligase i activity in lymphoblastoid cells from patients with bloom's syndrome
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5918217/
https://www.ncbi.nlm.nih.gov/pubmed/1900268
http://dx.doi.org/10.1111/j.1349-7006.1991.tb01745.x
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