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多功能蛋白聚糖剪接变体信使核糖核酸在正常人跟腱及肌腱病中的表达

Versican splice variant messenger RNA expression in normal human Achilles tendon and tendinopathies.

作者信息

Corps A N, Robinson A H N, Movin T, Costa M L, Ireland D C, Hazleman B L, Riley G P

机构信息

Rheumatology Research Unit, Box 194, Addenbrooke's Hospital, Cambridge CB2 2QQ, UK.

出版信息

Rheumatology (Oxford). 2004 Aug;43(8):969-72. doi: 10.1093/rheumatology/keh222. Epub 2004 May 11.

Abstract

OBJECTIVES

Versican is the principal large proteoglycan expressed in mid-tendon, but its role in tendon pathology is unknown. Our objective was to define the expression of versican isoform splice variant messenger ribonucleic acid (mRNA) in normal Achilles tendons, in chronic painful tendinopathy and in ruptured tendons.

METHODS

Total RNA isolated from frozen tendon samples (normal n = 14; chronic painful tendinopathy n = 10; ruptured n = 8) was assayed by relative quantitative reverse transcriptase polymerase chain reaction (RT-PCR) for total versican, versican variants V0, V1, V2, V3 and type I collagen alpha1 mRNA, normalized to glyceraldehyde-3-phosphate dehydrogenase (GAPDH). Differences between sample groups were tested by Wilcoxon statistics.

RESULTS

Painful and ruptured tendons showed a significant decrease (median 2-fold) in the expression of versican mRNA, in contrast to an increased expression (median 8-fold) of type I collagen alpha1 mRNA in painful tendons. Versican splice variants V0 and V1 mRNA were readily detected in normal samples, V3 levels were substantially lower, and V2 levels were more variable. Each of V1, V2 and V3 mRNA showed significant decreases in expression in painful and ruptured tendons, but V0 was not significantly changed.

CONCLUSIONS

Changes in versican expression relative to that of collagen, and alterations in the balance of versican splice variants, may contribute to changes in matrix structure and function in tendinopathies.

摘要

目的

多功能蛋白聚糖是肌腱中部表达的主要大型蛋白聚糖,但其在肌腱病理中的作用尚不清楚。我们的目的是确定多功能蛋白聚糖异构体剪接变异体信使核糖核酸(mRNA)在正常跟腱、慢性疼痛性肌腱病和断裂肌腱中的表达情况。

方法

从冷冻肌腱样本中分离出的总RNA(正常样本n = 14;慢性疼痛性肌腱病样本n = 10;断裂样本n = 8),通过相对定量逆转录聚合酶链反应(RT-PCR)检测总多功能蛋白聚糖、多功能蛋白聚糖变异体V0、V1、V2、V3和I型胶原α1 mRNA,并以甘油醛-3-磷酸脱氢酶(GAPDH)进行标准化。样本组间差异通过Wilcoxon统计检验。

结果

与疼痛性肌腱中I型胶原α1 mRNA表达增加(中位数8倍)相反,疼痛性和断裂肌腱中多功能蛋白聚糖mRNA表达显著降低(中位数2倍)。多功能蛋白聚糖剪接变异体V0和V1 mRNA在正常样本中易于检测到,V3水平显著较低,V2水平变化更大。V1、V2和V3 mRNA在疼痛性和断裂肌腱中的表达均显著降低,但V0无显著变化。

结论

多功能蛋白聚糖表达相对于胶原蛋白表达的变化,以及多功能蛋白聚糖剪接变异体平衡的改变,可能导致肌腱病中基质结构和功能的变化。

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