Subcellular Distribution of Axonally Transported Adenylate Cyclase: Effect of Nerve Constriction and Comparison with Acetylcholinesterase

Despite several studies indicating that cyclic nucleotides and their associated enzymes are present in peripheral nerves, their role in neuronal function remains unknown. One possible role is that of a modulating influence in the processes associated with axonal growth and maintenance, and in axonal regeneration. This study has used the frog sciatic nerve as a preparation for investigating the subcellular distribution of neuronai adenylate cyclase activity in normal and crush‐injured nerves. The experiments have focused primarily on the axonal transport of adenylate cyclase activity and its subcellular redistribution at the site of constriction. The adenylate cyclase activity measurements were also compared with similar measurements of acetylcholinesterase distribution. Adenylate cyclase activity in normal sciatic nerves increased in the segment proximal to a nerve constriction over time, but did not increase distal to the constriction. Subcellular fractionation of the accumulating activity indicated that the majority of axonally transported enzyme was associated with microsomal organelles; however, an additional transported component was found in the nuclear/mitochondrial fraction. The transport velocities of these two components were different. The microsomal activity appeared to be transported with Group I proteins, while the nuclear/mitochondrial activity was transported with Group II. Rapidly transported Group I proteins have been suggested to be destined principally for the axolemma or the agranular reticu‐lum, and the more slowly transported Group II proteins to be associated with intracellular organelles, including synaptic structures. Thus, axonally transported adenylate cyclase activity may have more than one functional role in peripheral nerve. The association of both adenylate cyclase and Protein I, an endogenous substrate for cyclic AMP, with Group II transport offers the intriguing possibility of a structural correspondence. Adenylate cyclase activity in Group I, however, did not appear to be transported with organelles which also contained acetylcholinesterase. The two enzymes, in terms of both velocity of transport and susceptibility to retrograde transport, were handled differently by the neuron. The subcellular distribution of adenylate cyclase activity in an isolated nerve segment was also found to change over time. Microsomal activity decreased, while nuclear/mitochondrial activity transiently increased and then also decreased. This may offer some indication of the morphological location of adenylate cyclase and its potential involvement in Wallerian degeneration and nerve regeneration, particularly in view of recent reports concerning the importance of local injury‐induced changes to the initiation of nerve regeneration. We have proposed a dynamic association between axonal calcium and cyclic AMP concentration, which provides a method for membrane renewal or degradation in the intact axon and may offer a molecular basis for the structural reorganization occurring in the proximal segment of an injured nerve.