Exogenous expression of an allatotropin-related peptide receptor increased the membrane excitability in Aplysia neurons

The neuropeptide allatotropin was first found in tissues of corpora allata in the insect Manduca sexta [7] and subsequently allatotropin-related peptides were characterized in Arthropoda, Annelida and Mollusca with various functions in different behaviors, including feeding. The allatotropin receptor was originally characterized in Bombyx mori [8], followed by identification of other insect allatotropin receptors, e.g., in Manduca sexta [9]. Additionally, two allatotropin receptors in the annelid Platynereis [10] and one in Aplysia [4] were characterized. Interestingly, phylogenetic analyses have shown that protostome allatotropin and deuterostome orexin signaling systems are orthologous [11].

In Aplysia, apATRP (GFRLNSASRVAHGY-NH2) acts on the feeding motor circuit to enhance motor neuron B61/62 excitability. This increases B61/62 firing frequency, thereby compensating for the short duration of B61/62 bursts during feeding motor programs elicited by an apATRP-positive command neuron [2]. B61/62 firing frequency also increases after learning that food is inedible [12]. Recently, several ligands, including apATRP, were found to activate apATRPR in CHO-K1 cells transiently transfected with apATRPR. Importantly, the pattern of activations of these ligands in the cell line matches their actions on B61/62 excitability, suggesting that apATRPR likely functions in the Aplysia CNS [4]. However, it is unknown whether apATRPR mediates the excitability increase in native Aplysia neurons, given that there might be multiple apATRP receptors in Aplysia. Here, we sought to determine whether apATRP is sufficient to mediate the ligand effect on native neurons by evaluating the ability of apATRP to activate apATRPR in Aplysia neurons that do not endogenously express apATRPR. To express apATRPR in neurons, we used a plasmid vector, pNEX3, which is an effective method to express exogenous proteins in cultured Aplysia neurons [5, 6]. Thus, we constructed the recombinant plasmid pNEX3-apATRPR (Additional file 1).

To demonstrate that apATRPR might function as an endogenous receptor of apATRP, we first sought to find a target neuron that did not natively express apATRPR in the buccal ganglia. We selected a larger neuron, B8 (~ 150 μm), and examined B8 excitability changes in response to apATRP. apATRP increased B8 excitability (Fig. 1a, b), suggesting that B8 might contain a receptor(s) for apATRP. Therefore, B8 neurons were excluded. After testing several additional neurons, we found that another large neuron B1/B2 (~ 210 μm) did not respond to apATRP (Fig. 1c, d), and it was used as the target neuron.

apATRP increased the excitability of B1/B2 neurons that were exogenously expressed with the receptor apATRPR. a, b apATRP increased B8 excitability at 10^–5 M but not at 10^–6 M (F(3, 6) = 14.89, p < 0.01, n = 3 individual neurons from three preparations). Bonferroni post hoc tests: *p < 0.05, **p < 0.01. Error bars, SE. c, d apATRP had no significant effect on B1/B2 excitability (F(3, 9) = 1.00, p > 0.05, n = 4 individual neurons from four preparations). Error bars, SE. e The caudal surface of a buccal ganglion viewed with a regular light source. B1/B2 and other neurons on the left side were microinjected with plasmids pNEX3-apATRPR and pNEX3-EGFP, and B1/B2 and other neurons on the right side were microinjected with only plasmid pNEX3-EGFP. Arrows indicate the neurons injected with plasmids and expressed the EGFP protein (showed bright fluorescence under a fluorescence microscope, see panel f). Arrowheads indicate the neurons injected with plasmids but did not express the EGFP protein. f B1/B2 neurons on both sides showed bright fluorescence (green, arrows) under a fluorescence microscope. The left B1/B2 neuron expressed apATRPR and EGFP, and the right B1/B2 neuron expressed EGFP. Other neurons marked with arrowheads in (e) did not express injected genes. g, h A magnified view of the injected neurons in (f) showing left B1/B2 neuron (g) and right B1/B2 neuron (h). Scale bar in f: 500 μm (scale bar in f is for e and f); Scale bar in h: 200 μm (scale bar in h is for g and h). i, j At 10^–6 M and 10^–5 M, apATRP increased B1/B2 excitability (F(3, 9) = 44.84, p < 0.0001, n = 4 individual neurons from three preparations), which expressed the receptor apATRPR. Bonferroni post hoc tests: ***p < 0.001. Error bars, SE. k, l apATRP had no significant effects on B1/B2 neurons that do not express the receptor apATRPR (F(3, 6) = 1.60, p > 0.05, n = 3 individual neurons from three preparations). Bars in a, c, i and k denote current injections. Control groups and wash groups in a, c, i, k were perfused with high divalent saline only, whereas the experimental groups in a, c, i, k were perfused with the neuropeptide apATRP dissolved in high divalent saline

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In each hemi-ganglion of the buccal ganglion, there are one B1 and one B2 neuron. Thus, there are four B1/B2 neurons on both sides of the buccal ganglion. We set up two groups: the plasmid pNEX3-EGFP mixture with fast green microinjected into B1/B2 neurons as the control group, and the plasmid pNEX3-EGFP and pNEX3-apATRPR mixture with fast green microinjected into the contralateral B1/B2 neurons as the experimental group. Visualizing fast green with a regular light source confirmed that the plasmid injection was successful (Fig. 1e). After injection, we placed the buccal ganglion into cell culture until we observed that B1/B2 neurons exhibited green fluorescence (Fig. 1f–h), which took 1 to 3 days. Observing green fluorescence confirmed that neurons had expressed the EGFP in the control group and had co-expressed the apATRPR and EGFP in the experimental group.

We next perfused apATRP into the recording dish and tested B1/B2 excitability. The results showed that B1/B2 excitability in the experimental group was enhanced (Fig. 1i, j), and B1/B2 excitability in the control group showed no significant changes (Fig. 1k, l). This finding indicated that the neuropeptide receptor, apATRPR, could mediate the excitability increase in native Aplysia neurons in response to its ligand, apATRP.

In this work, we have characterized physiological functions of a neuropeptide receptor, apATRPR, expressed in Aplysia neurons. Our study provides a definitive evidence that apATRPR indeed mediates excitability increase in a neuron that does not express apATRPR, indicating that the neuropeptide receptor, apATRPR, is sufficient to mediate an excitability increase to its ligand, apATRP, in Aplysia neurons. In terms of molecular mechanisms underlying the excitability increase, we speculate that, similar to insects [9], through Gαs, apATRPR could increase cAMP, which could in turn act either to close K channels through PKA [13] or to activate cAMP-gated Na channels through a PKA-independent pathway (Additional file 1).

Taken together with earlier work showing that pNEXδ or pNEX3 can express GPCRs for glutamate, octopamine and serotonin [13,14,15], pNEX, including pNEXδ and pNEX3, proves to be an effective plasmid to express GPCRs for both small molecule transmitters and neuropeptides in Aplysia neurons. We expect that such a procedure could be readily applied to demonstrate physiological functions of neuropeptide receptors in native neurons in model systems with reasonably large identifiable neurons, such as other molluscs, annelids and possibly some arthropods. Notably, compared with invertebrate organisms such as C. elegans and Drosophila, life spans of molluscs and annelids are relatively long and life cycles are complex, making it difficult to use transgenes to manipulate gene expression. Consequently, the procedure described in this paper should be particularly useful in these animals to study functions of genes in native neurons.