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通过逆转录聚合酶链反应(RT-PCR)对小鼠膝关节关节囊和关节软骨中mRNA水平进行定量:关节炎期间基质溶解素和白细胞介素-1 mRNA水平的动力学变化

Quantification of mRNA levels in joint capsule and articular cartilage of the murine knee joint by RT-PCR: kinetics of stromelysin and IL-1 mRNA levels during arthritis.

作者信息

Van Meurs J B, Van Lent P L, Joosten L A, Van der Kraan P M, Van den Berg W B

出版信息

Rheumatol Int. 1997;16(5):197-205. doi: 10.1007/BF01330296.

Abstract

We developed a method to isolate well defined joint specimens from different compartments of normal and arthritic murine knee joints in which mRNA levels of stromelysin and IL-1 were semiquantified using RT-PCR. Joint capsule specimens were isolated on medial and lateral sides of the patella with a biopsy punch. Cartilage layers were isolated from patellae after a mild decalcification with EDTA. EDTA treatment had no effect on the amount and efficiency of amplification of mRNA when tested on isolated chondrocytes. After induction of experimental arthritis, stromelysin mRNA was elevated approximately 50 times in both joint capsule and cartilage. IL-1 was elevated 100 times in joint capsule but only 10 times in cartilage. Kinetic analysis of mRNA levels in cartilage during arthritis showed a prolonged elevation of stromelysin mRNA compared to IL-1. The variation in mRNA levels between joints of individual mice proved to be low, showing that sampling of the specimens and subsequent RT-PCR can be performed reliably. The current method offers a valuable approach to study gene expression in knee joints during murine experimental arthritis.

摘要

我们开发了一种方法,可从正常和患有关节炎的小鼠膝关节的不同腔室中分离出明确的关节标本,其中使用逆转录聚合酶链反应(RT-PCR)对基质溶解素和白细胞介素-1(IL-1)的mRNA水平进行半定量分析。使用活检打孔器在髌骨的内侧和外侧分离关节囊标本。用乙二胺四乙酸(EDTA)轻度脱钙后,从髌骨中分离软骨层。在分离的软骨细胞上进行测试时,EDTA处理对mRNA的扩增量和效率没有影响。诱导实验性关节炎后,关节囊和软骨中的基质溶解素mRNA均升高约50倍。IL-1在关节囊中升高100倍,但在软骨中仅升高10倍。对关节炎期间软骨中mRNA水平的动力学分析表明,与IL-1相比基质溶解素mRNA升高的时间更长。事实证明,个体小鼠关节之间mRNA水平的差异很小,这表明标本采样和随后的RT-PCR可以可靠地进行。目前的方法为研究小鼠实验性关节炎期间膝关节中的基因表达提供了一种有价值的方法。

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