Identification of agrin, a synaptic organizing protein from Torpedo electric organ.

Nitkin, Ralph; Smith, Martin A.; Magill, Catherine; Fallon, Justin R.; Yao, Yung-Mae; Wallace, Bruce G.; McMahan, Uel J.

doi:10.1083/jcb.105.6.2471

Cited by 447 publications

(297 citation statements)

References 43 publications

(64 reference statements)

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“…Agrn is an essential component of the basal lamina within the neuromuscular junction, where its organizational role is well understood (Nitkin et al, 1987). We detected Agrn in our synaptosomal preparations confirming its presence in the central nervous system synapse.…”

Section: Discussionsupporting

confidence: 72%

Cerebral Ischemia Causes Dysregulation of Synaptic Adhesion in Mouse Synaptosomes

Costain

Rasquinha

Sandhu

et al. 2007

J Cereb Blood Flow Metab

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Synaptic pathology is observed during hypoxic events in the central nervous system in the form of altered dendrite structure and conductance changes. These alterations are rapidly reversible, on the return of normoxia, but are thought to initiate subsequent neuronal cell death. To characterize the effects of hypoxia on regulators of synaptic stability, we examined the temporal expression of cell adhesion molecules (CAMs) in synaptosomes after transient middle cerebral artery occlusion (MCAO) in mice. We focused on events preceding the onset of ischemic neuronal cell death ( < 48 h). Synaptosome preparations were enriched in synaptically localized proteins and were free of endoplasmic reticulum and nuclear contamination. Electron microscopy showed that the synaptosome preparation was enriched in spheres (E650 nm in diameter) containing secretory vesicles and postsynaptic densities. Forebrain mRNA levels of synaptically located CAMs was unaffected at 3 h after MCAO. This is contrasted by the observation of consistent downregulation of synaptic CAMs at 20 h after MCAO. Examination of synaptosomal CAM protein content indicated that certain adhesion molecules were decreased as early as 3 h after MCAO. For comparison, synaptosomal Agrn protein levels were unaffected by cerebral ischemia. Furthermore, a marked increase in the levels of p-Ctnnb1 in ischemic synaptosomes was observed. p-Ctnnb1 was detected in hippocampal fiber tracts and in cornu ammonis 1 neuronal nuclei. These results indicate that ischemia induces a dysregulation of a subset of synaptic proteins that are important regulators of synaptic plasticity before the onset of ischemic neuronal cell death.

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Section: Discussionsupporting

confidence: 72%

Cerebral Ischemia Causes Dysregulation of Synaptic Adhesion in Mouse Synaptosomes

Costain

Rasquinha

Sandhu

et al. 2007

J Cereb Blood Flow Metab

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“…Native agri n has been best characterized in basal lamina extracts of the electric o rgan of the ray T. californica. The extracts contain two forms of agrin, 150 and 95 kd, both of which have AChR/AChE aggregating activity (Nitkin et al, 1987). Both proteins are likely to be derived from a larger protein that is proteolytically cleaved either during tissue extraction or during in situ posttranslational modification; the 95 kd form is located in the C-terminal half of the large protein (Smith et al, submitted; Tsim et al, 1992).…”

Section: Discussionmentioning

confidence: 99%

“…After overnight incubation at 4°C, 100 !ll of a 1:1 suspension of protein A-Sepharose beads (Pharmacia) was added, and the incubation was continued for 2 hr at room temperature. Beads were pelleted by centrifugation and washed sequentially as described in Nitkin et al (1987). Bound antigen-antibody complexes were released by boiling for 5 min in 60 !ll of SDS-polyacrylamide gel electrophoresis sam pie buffer (3% SDS, 5% 2-mercaptoethanol, 15% glycerol, 0.001% brom phenol blue in 62.5 mM Tris-HCI [pH 6.5]).…”

Section: Immunoprecipitations and Gel Electrophoresismentioning

confidence: 99%

“…However, basal lamina at nonsynaptic sites in a variety of tissues including muscle, central nervous system (CNS), heart, and kidney, where AChRs and AChE are not known to aggregate, is also stained by these antibodies (Reist et al, 1987;Godfrey et al, 1988aGodfrey et al, , 1988b. Moreover, proteins inactive in AChR aggregation assays are immunoprecipitated from extracts of several different tissues by antiagrin MAbs (Nitkin et al, 1987;Godfrey, 1991). Such findings have led to the suggestion that anti-agrin MAbs also recognize proteins other than agrin and that these proteins differ from agrin in their function.…”

Section: Introductionmentioning

confidence: 99%

“…Transfection experiments revealed that the proteins encoded by these cDNAs are recognized by anti-agrin antibodies, but unlike agrin, they are inactive in standard AChR aggregation assays. Because the discovery of agrin was based on its ability to cause AChRs to aggregate in cultured chick myotubes (Godfrey et al, 1984;Nitkin et al, 1987) and because the two proteins we describe here lack the AChR aggregating activity, but are highly similarto agrin in structure, we refer to them simply as agrin-related proteins 1 and 2 (ARP-1 and ARP-2). The predicted amino acid sequences of the agrin-related proteins are identical to that of agrin except for the absence of a stretch of 11 amino acids in ARP-1 and stretch es of the 11 and 4 amino acids in ARP-2.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

The agrin gene codes for a family of basal lamina proteins that differ in function and distribution

Rüegg

Tsim

Horton

et al. 1992

Neuron

238

198

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SummaryWe isolated two cDNAs that encode isoforms of agrin, the basal lamina protein that mediates the motor neuron-induced aggregation of acetylcholine receptors on muscle fibers at the neuromuscular junction. 80th proteins are the result of alternative splicing of the product of the agrin gene, but, unlike agrin, they are inactive in standard acetylcholine receptor aggregation assays. They lack one (agrin-related protein 1) or two (agrinrelated protein 2) regions in agrin that are required for its activity. Expression studies provide evidence that both proteins are present in the nervous system and muscle and that, in muscle, myofibers and Schwann cells synthesize the agrin-related proteins while the axon terminals of motor neurons are the sole source of agrin.

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Distribution and substrate properties of agrin, a heparan sulfate proteoglycan of developing axonal pathways

et al. 1997

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The distribution and substrate properties of agrin, an extracellular matrix heparan sulfate proteoglycan (HSPG), was investigated in the developing chick nervous system by immunocytochemistry, Western blotting, and in neurite outgrowth assays. By comparing the distribution of agrin with that of laminin-1, merosin (laminin-2), neurofilament, and neural cell adhesion molecule (NCAM), it was found that throughout development, agrin is a constituent of all basal laminae. From embryonic day (E) 4 onwards, agrin is also abundant in axonal pathways of the central nervous system, such as the optic nerve, the tectobulbar pathway, the white matter of the spinal cord, and the marginal and the molecular layers of the forebrain and the cerebellum. The abundance of agrin in brain decreases from E13 onwards. In the peripheral nervous system, agrin is present throughout development as a constituent of the Schwann cell basal laminae. Western blots confirmed the immunocytochemical data, showing maximum expression of agrin occurs during the early to medium stages of brain development. Western blots also showed that in mouse and human brain, agrin exists as an HSPG. Purified agrin did not support neurite outgrowth, rather it inhibited retinal neurite extension on mixed agrin/merosin substrates. Despite the fact that agrin, when used as a substrate inhibited neurite outgrowth, its temporal and spatial overlap with growing axons suggests that agrin has a supportive role in the development of axonal pathways, possibly as a binding component for growth factors and cell adhesion proteins.

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Identification of agrin, a synaptic organizing protein from Torpedo electric organ.

Cited by 447 publications

References 43 publications

Cerebral Ischemia Causes Dysregulation of Synaptic Adhesion in Mouse Synaptosomes

Cerebral Ischemia Causes Dysregulation of Synaptic Adhesion in Mouse Synaptosomes

The agrin gene codes for a family of basal lamina proteins that differ in function and distribution

Distribution and substrate properties of agrin, a heparan sulfate proteoglycan of developing axonal pathways

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