Wright John W, Brown Travis E, Harding Joseph W
Department of Psychology, Washington State University, Pullman, WA 99164-4820, USA.
Neural Plast. 2007;2007:73813. doi: 10.1155/2007/73813. Epub 2006 Dec 14.
Memory consolidation requires synaptic reconfiguration dependent upon extracellular matrix (ECM) molecules interacting with cell adhesion molecules. Matrix metalloproteinase (MMP) activity is responsible for transient alterations in the ECM that may be prerequisite to hippocampal-dependent learning. In support of this hypothesis we have measured increases in MMP-3 and MMP-9 levels within the hippocampus and prefrontal cortex during Morris water maze training. The present investigation extends these findings by determining that infusion of an MMP inhibitor (FN-439) into the dorsal hippocampus disrupted acquisition of this task. In vitro fluorescence enzyme assays to determine the specificity of FN-439 against the catalytic domains of MMP-3 and MMP-9 indicated mean +/- SEM IC(50)s of 16.2 +/- 7.8 and 210.5 +/- 37.8 muM, respectively, while in situ zymography using hippocampal sections treated with FN-439 indicated significant reductions in MMP gelatinase activity. These results suggest that compromising the ability of the dorsal hippocampus to reconfigure ECM molecules by inhibiting MMP activity interferes with appropriate spatial memory acquisition, and support a role for hippocampal MMPs in the phenomena of spatial memory acquisition and storage.
记忆巩固需要依赖细胞外基质(ECM)分子与细胞黏附分子相互作用的突触重构。基质金属蛋白酶(MMP)的活性负责ECM的短暂改变,这可能是海马体依赖学习的先决条件。为支持这一假设,我们在莫里斯水迷宫训练期间测量了海马体和前额叶皮质内MMP-3和MMP-9水平的升高。本研究通过确定向背侧海马体注射MMP抑制剂(FN-439)会破坏该任务的习得,扩展了这些发现。用于确定FN-439对MMP-3和MMP-9催化结构域特异性的体外荧光酶分析表明,平均±标准误IC(50)分别为16.2±7.8和210.5±37.8μM,而使用经FN-439处理的海马体切片进行的原位酶谱分析表明MMP明胶酶活性显著降低。这些结果表明,通过抑制MMP活性来损害背侧海马体重构ECM分子的能力会干扰适当的空间记忆习得,并支持海马体MMP在空间记忆习得和存储现象中的作用。