The stomatogastric nervous system (STNS) of adult lobsters and crabs generates a number of different rhythmic motor patterns which control different regional movements of the foregut. Since these output patterns are generated by discrete neural networks that, in the adult, are well characterized in terms of synaptic and cellular properties, this system constitutes an ideal model for exploring the mechanisms underlying the ontogeny of neural network organization. The foregut and its rhythmic motor patterns were studied in in vitro STNS nerve-muscle preparations of the embryo and different larval stages of the lobster Homarus gammarus. The development of Homarus comprises a long embryonic stage in ovo followed by three pelagic larval stages prior to the onset of benthic life. During these stages the foregut itself develops slowly from a simple ectodermal invagination that occurs in the embryo. During successive larval stages it progressively acquires all the specialized structures and shape of the adult foregut. In contrast, the STNS is morphologically recognizable at early embryonic stages. In all recorded stages the STNS spontaneously expresses rhythmic motor activity. During development, this activity is progressively restructured, beginning with a single rhythmic motor pattern in the embryo where all the stomodeal muscles are strongly coordinated. In subsequent stages, however, this single pattern is progressively subdivided to give rise eventually to the three discrete rhythmic motor patterns characteristic of the adult STNS. Our data suggest that rather than a dismantling of redundant embryonic and larval neural networks, the different adult networks emerge as a progressive partitioning of discrete circuits from a single embryonic network.
In the adult lobster, Homarus gammarus, the stomatogastric ganglion (STG) contains two well-defined motor pattern generating networks that receive numerous modulatory peptidergic inputs from anterior ganglia. We are studying the appearance of extrinsic peptidergic inputs to these networks during ontogenesis. Neuron counts indicate that as early as 20% of development (E20) the STG neuronal population is quantitatively established. By using immunocytochemical detection of 5-bromo-2'-deoxyuridine incorporation, we found no immunopositive cells in the STG by E70. We concluded that the STG neuronal population remains quantitatively stable from mid-embryonic life until adulthood. We then investigated the ontogeny of FLRFamide- and proctolin-like peptides in the stomatogastric nervous system, from their first appearance until adulthood by using whole mount immunocytochemistry. Numerous FLRFamide-like-immunoreactive STG neuropilar ramifications were observable as early as E45 and remain thereafter. From E50 to the first larval stage, one to three STG somata stained, while somatic staining was not observed in larval stage II and subsequent stages. From E50 and thereafter, the STG neuropilar area was immunopositive for proctolin. One to two proctolinergic somata were detected in the STG of the three larval stages but were not seen in embryos, the post-larval stage or in adults. Thus, peptidergic inputs to the STG are present from mid-embryonic life. Moreover, whereas in the adult, STG neurons only contain glutamate or acetylcholine, some neurons transiently express peptidergic phenotypes during development. Although this system expresses an ontogenetic peptidergic plasticity, the STG neurons produce a single stable embryonic-larval motor output (Casasnovas and Meyrand [1995] J. Neurosci. 15:5703-5718).
Dopamine-immunoreactive neurons were revealed in lobster embryos, larvae, and postlarvae, and staining patterns were compared to neuronal labeling in the juvenile lobster nervous system (Cournil et al. [1994] J. Comp. Neurol. 344:455-469). Dopamine immunoreactivity is first detected by midembryonic life in 35-40 neuronal somata located anteriorly in brain and subesophageal ganglion. When the lobsters assume a benthic life during the first postlarval stage, an average of 58 cell bodies are labeled. The acquisition of dopamine in lobster neurons is a protracted event spanning embryonic, larval, and postlarval life and finally reaching the full complement of roughly 100 neurons in juvenile stages. Some of the dopaminergic neurons previously identified in the mature nervous system, such as the paired Br cells, L cells, and mandibular cells, are labeled in embryos and persist throughout development. In contrast, other neurons stain transiently for dopamine during the developmental period, but, by the adult stage, these neurons are no longer immunoreactive. Such transiently labeled neurons project to the foregut, the thoracic dorsal muscles, the neurohormonal pericardial plexus, and the pericardial pouches. It is proposed that these neurons are alive and functioning in adult lobster but that dopamine levels have been abolished, providing that neurotransmitter status is a dynamic, changing process.
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