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小鼠溶菌酶M和P的杀菌活性与溶菌酶活性比较。

Comparison of the microbicidal and muramidase activities of mouse lysozyme M and P.

作者信息

Markart Philipp, Faust Nicole, Graf Thomas, Na Cheng-Lun, Weaver Timothy E, Akinbi Henry T

机构信息

Zentrum für Innere Medizin, Medizinische Klinik II, Klinikstrasse 36, 35392 Giessen, Germany.

出版信息

Biochem J. 2004 Jun 1;380(Pt 2):385-92. doi: 10.1042/BJ20031810.

Abstract

Lysozyme is one of the most abundant antimicrobial proteins in the airspaces of the lung. Mice express two lysozyme genes, lysozyme M and P, but only the M enzyme is detected in abundance in lung tissues. Disruption of the lysozyme M locus significantly increased bacterial burden and mortality following intratracheal infection with a Gram-negative bacterium. Unexpectedly, significant lysozyme enzyme activity (muramidase activity) was detected in the airspaces of uninfected lysozyme M-/- mice, amounting to 25% of the activity in wild-type mice. Muramidase activity in lysozyme M-/- mice was associated with increased lysozyme P mRNA and protein in lung tissue and bronchoalveolar lavage fluid respectively. The muramidase activity of recombinant lysozyme P was less than that of recombinant M lysozyme. Recombinant P lysozyme was also less effective in killing selected Gram-negative bacteria, requiring higher concentrations than lysozyme M to achieve the same level of killing. The lower antimicrobial activity of P lysozyme, coupled with incomplete compensation by P lysozyme in lysozyme M-/- mice, probably accounts for the increased susceptibility of null mice to infection. Recombinant lysozyme M and P were equally effective in killing selected Gram-positive organisms. This outcome suggests that disruption of both M and P loci would significantly increase susceptibility to airway infections, particularly those associated with colonization by Gram-positive organisms.

摘要

溶菌酶是肺气道中含量最丰富的抗菌蛋白之一。小鼠表达两种溶菌酶基因,即溶菌酶M和P,但在肺组织中大量检测到的只有M酶。溶菌酶M基因座的破坏显著增加了气管内感染革兰氏阴性菌后的细菌负荷和死亡率。出乎意料的是,在未感染的溶菌酶M基因敲除小鼠的气道中检测到显著的溶菌酶活性(胞壁质酶活性),相当于野生型小鼠活性的25%。溶菌酶M基因敲除小鼠的胞壁质酶活性分别与肺组织和支气管肺泡灌洗液中溶菌酶P的mRNA和蛋白增加有关。重组溶菌酶P的胞壁质酶活性低于重组M溶菌酶。重组P溶菌酶在杀死选定的革兰氏阴性菌方面也效果较差,需要比溶菌酶M更高的浓度才能达到相同的杀伤水平。P溶菌酶较低的抗菌活性,加上溶菌酶M基因敲除小鼠中P溶菌酶的不完全补偿,可能是基因敲除小鼠对感染易感性增加的原因。重组溶菌酶M和P在杀死选定的革兰氏阳性菌方面同样有效。这一结果表明,M和P基因座的破坏将显著增加对气道感染的易感性,特别是那些与革兰氏阳性菌定植相关的感染。

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