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The Journal of Neuroscience, September 3, 2003, 23(22):8159-8166
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Mutations in deadly seven/notch1a Reveal Developmental Plasticity in the Escape Response Circuit
Katharine S. Liu,1 * Michelle Gray,2,3 * Stefanie J. Otto,1 Joseph R. Fetcho,1 andChristine E. Beattie2,3,4 1Department of Neurobiology, State University of New York at Stony Brook, Stony Brook, New York 11794, 2Center for Molecular Neurobiology, 3Molecular, Cellular, and Developmental Biology Program, and 4Department of Neuroscience, The Ohio State University, Columbus, Ohio 43210
Abstract
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Abstract
Introduction
The relatively simple neural circuit driving the escape response in zebrafish offers an excellent opportunity to study properties of neural circuit formation. The hindbrain Mauthner cell is an essential component of this circuit. Mutations in the zebrafish deadly seven/notch1a (des) gene result in supernumerary Mauthner cells. We addressed whether and how these extra cells are incorporated into the escape-response circuit. Calcium imaging revealed that all Mauthner cells in desb420 mutants were active during an elicited escape response. However, the kinematic performance of the escape response in mutant larvae was very similar to wild-type fish. Analysis of the relationship between Mauthner axon collaterals and spinal neurons revealed that there was a decrease in the number of axon collaterals per Mauthner axon in mutant larvae compared with wild-type larvae, indicative of a decrease in the number of synapses formed with target spinal neurons. Moreover, we show that Mauthner axons projecting on the same side of the nervous system have primarily nonoverlapping collaterals. These data support the hypothesis that excess Mauthner cells are incorporated into the escape-response circuit, but they divide their target territory to maintain a normal response, thus demonstrating plasticity in the formation of the escape-response circuit. Such plasticity may be key to the evolution of the startle responses in mammals, which use larger populations of neurons in circuits similar to those in the fish escape response.
Key words: hindbrain; behavior; calcium imaging; mutant analysis; Mauthner cell; notch1a; axon collaterals
Introduction
Establishing functional neural circuits involves numerous developmental processes, including the generation of the correct cell number and cell type and the establishment of appropriate connections between cells. Mutations that alter these processes have the potential to disrupt the relationship between cell types in a circuit and can compromise downstream behavior, unless the animal can adapt to such changes. Zebrafish offer several advantages as a model system for studying the impact of mutations on circuitry and behavior. In aquatic vertebrates, such as fish and premetamorphic amphibians, relatively simple neural circuits control fundamental motor behaviors. These circuits often have relatively few cells, and, in some cases, it is possible to identify individual cells and link them to a behavior. This is particularly true in the zebrafish hindbrain, in which there is an array of morphologically distinct reticulospinal neurons with characteristic cell body locations and stereotyped axon projections (Metcalfe et al., 1986). The largest of these, the Mauthner cell, is present bilaterally in rhombomere segment 4 and sends its axon across the midline where it descends to make monosynaptic connections with contralateral interneurons and motoneurons along the length of the spinal cord (Faber and Korn, 1978
Mutations in the des/notch1a gene (van Eeden et al., 1996
Materials and Methods
Fish care and identification. Mutant embryos and larvae were obtained from a laboratory breeding stock of heterozygous adult fish. Homozygote mutants were obtained from natural mating of heterozygous adults and were identified by their somitic defect that results in irregular muscle patterns. Both the b420 and tp37 allele carry ethylnitrosourea-induced mutations (van Eeden et al., 1996Whole-mount antibody labeling. Whole-mount antibody labeling with 3A10 antibody (1/10; Developmental Studies Hybridoma Bank, University of Iowa, Iowa City, IA) and acetylated tubulin (1/400; Sigma, St. Louis, MO) were processed as described by Gray et al. (2001
Retrograde labeling of calcium green dextran. Larval zebrafish were anesthetized with 0.02% 3-aminobenzoic acid ethyl ester (MS222, tricaine). The targeted cells were retrogradely labeled by pressure injection via a glass microelectrode of a 50% solution of calcium green dextran [10,000 molecular weight (MW); Molecular Probes, Eugene, OR) in 10% HBSS into the caudal spinal cord (Fetcho and O'Malley, 1995
Calcium imaging. Calcium imaging was performed as described previously (Fetcho and O'Malley, 1995
Escapes were elicited by a small tap from a polished glass probe attached to a piezoelectric crystal. The stimulus (tap) strength could be controlled by the amount of voltage applied to the crystal. Taps given to the head were aimed at the ear of the animal, ipsilateral to the group of cells under observation. Taps given to the tail were aimed rostral of the injection site and ipsilateral to the observed cells.
The fluorescence intensities of the cells were monitored by collecting a baseline series of images of a group of labeled Mauthner cells at 300 msec intervals before delivering the stimulus. To avoid false positives resulting from the cells moving to a brighter plane of focus, we started with the brightest plane of focus, optimizing for one cell at a time per trial. Although the optimized cell increased in fluorescence intensity, in most cases, the surrounding Mauthner cells could be seen to brighten as well.
High-speed recording of behavior. High-speed recording was performed as described previously (Liu and Fetcho, 1999
Fish were tapped on the left side of the head for the first trial, on the right side of the head for the second trial, and then the left side of the tail for the third trial, and so on. Stimuli to the head were directed at the ear, whereas stimuli to the tail were directed caudal to the anal pore. All fish in the group were tested for the same quadrant before moving on to the next trial, resulting in each fish resting for an average of 20 min between trails, and each fish was not presented with a stimulus in the same quadrant for well over 1 hr. Such delays should prevent habituation, fatigue, etc. On occasion, a fish failed to respond to the stimulus, gave a premature response, or turned slightly on its side. Only responses that occurred after the stimulus were deployed, and in which the fish remained upright throughout the initial bend were kept digitally. Because desb420 homozygotes do not develop a swim bladder, we chose to collect our trials at 3 dpf, when neither wild-type larvae nor desb420 larvae have swim bladders.
Data analysis. Analyses of the recorded movement data were done as described previously (Liu and Fetcho, 1999
Single Mauthner axon labels. Mauthner axons of 3 dpf larvae, anesthetized in tricaine, were retrogradely labeled by pressure injection into the spinal cord using a glass electrode filled with 5% lysinated rhodamine dextran (10,000 MW) (all fluorescent dextrans used in this study were obtained from Molecular Probes) at approximately hemisegment 25. After labeling, larvae were allowed to recover for 24 hr. Because of the difficulty in resolving multiple fluorescent-labeled axons in desb420 mutants, only larvae with one labeled Mauthner axon were scored. Collaterals were imaged and counted under confocal microscopy (63x) over a three-somite length corresponding to three spinal cord hemisegments. The total number of Mauthner cells present on the corresponding side of the hindbrain was quantitated on a Zeiss Axioplan compound microscope under transmitted light (40x).
Dual-color Mauthner axon labels. Mauthner cells of 4 dpf larvae, anesthetized in tricaine, were retrogradely labeled by pressure injection into the spinal cord using a glass electrode filled with 10% fluorescein dextran (3000 MW). After a recovery of 48 hr, fish were screened for labeled Mauthner cells. These fish were anesthetized again, placed on a cover glass in a Petri dish, and embedded upright (dorsal side up) in a layer of 1.2% agar. Mauthner cells were targeted for electroporation under FITC fluorescence. For electroporation, thin-walled filamented glass microelectrodes backfilled with either 10% rhodamine dextran (3000 MW) or 10% Alexa 647 (10,000 MW) were used to electroporate single Mauthner cells (Haas et al., 2002
Results
The escape response circuit in desb420 mutants
The neural circuit driving the escape response in zebrafish is mediated by a defined set of neurons. Sensory input from the trigeminal (V) cranial nerve, acoustic (VIII) cranial nerve, and lateral line contact the Mauthner cell lateral dendrite (Kimmel et al., 198119% increase in primary motoneurons in desb420 mutants, whereas all other cells in the escape-response circuit appeared unaffected (Gray et al., 2001
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Figure 1. des mutants have supernumerary Mauthner cells. A, B, Mauthner cells in a 30 hr wild-type (A) and desb420 (B) mutant embryo as revealed by 3A10 antibody labeling and confocal microscopy. Dorsal views with anterior to the top. Scale bar, 40 µm.
Supernumerary Mauthner cells are active during the escape response
The presence of excess Mauthner cells in desb420 mutants prompted us to ask whether all of these cells participated in the escape response. Taking advantage of the transparency of zebrafish larvae, we used optical imaging of calcium-dependent fluorescent indicators to monitor the activity of several cells simultaneously (O'Malley et al., 1996Data were collected from 21 escape trials (17 to tail and 4 to head) from six fish. Figure 2 shows an example of a calcium-imaging trial. In this case, four cells were labeled on the side being imaged (Fig. 2A, arrow), and the change in fluorescence intensities was quantified (Fig. 2B,C). Because of potential movement artifacts, each calcium-imaging trial began at the brightest plane of focus for the cell of interest (Fetcho and O'Malley, 1995
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Figure 2. Mauthner cells in des mutants are active during an escape response. A calcium-imaging trial of a desb420 mutant is shown. A, Mauthner cells in mutant larvae were backfilled with the fluorescent dye, calcium green dextran, at 4 dpf and imaged on confocal microscopy with a 63x objective. B, For quantification purposes, Mauthner cells on the right side of the hindbrain (A, arrow) were numbered 1 through 4. Fluorescence intensities were presented in pseudocolor with red being the brightest. In this trial, the plane of focus was optimized for cell 3. However, as is typically the case, all four cells were noticeably brighter after the escape when compared with the baseline of frames collected before the stimulus. The distortion in frame 6 indicates movement of the fish in response to a tap on the tail. Frames are ordered from left to right with 578 msec between frames. C, Quantification of the increase in fluorescence intensities. The fluorescence intensities for each cell (1-4) were plotted for each frame. The y-axis shows the normalized intensities ( F/F). The x-axis shows the time in seconds. Scale bar, 30 µm.
The observation that all of the Mauthner cells responded to the stimulus might be a consequence of a strong stimulus that was suprathreshold for all cells, or it might be a result of mutual excitation among the cells via gap junctions or other synaptic interactions. To attempt to distinguish between these two possibilities, we repeated the calcium-imaging experiments while lowering the stimulus intensity to threshold, which is the intensity at which the fish escapes 50% of the time when presented with the stimulus. If Mauthner cells were independently activated by the sensory inputs, we might expect that near threshold for the behavior, some cells would fire and not others because of slight differences in the level of sensory input or threshold of the cells that would bring some cells to threshold and not others. The threshold stimulus intensity was determined for a mutant fish by varying the tap strength to find a strength at which the fish escaped to
Mauthner cells are contacted presynaptically on the Mauthner cell lateral dendrite by the trigeminal, acoustic, and lateral line nerves (Kimmel et al., 1990
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Figure 3. Mauthner cell lateral dendrites in des mutants are in close apposition to sensory nerves. A-D, Seventy-two hour wild-type (A, C) and mutant (B, D) embryos were labeled with 3A10 antibody and analyzed by confocal microscopy. The trigeminal (Tg) and lateral line (Ll) nerves extend perpendicular to the Mauthner cell (Mth) and are closely juxtaposed to Mauthner cell lateral dendrites (arrow). A and B are the left sides of merged sections of wild-type and mutant embryos; C and D are single optical sections through the wild-type and mutant embryo shown in A and B. All images are dorsal views with anterior to the top. Scale bar, 35 µm
Escape performance is similar in wild-type and desb420 mutant larvae
The Mauthner cell is known to play a major role in escape performance, particularly in tail-elicited escapes (Liu and Fetcho, 1999To compare the escape performance of desb420 mutants with wild-type animals, we captured escape responses with a high-speed (1000 frames per second) digital camera (Fig. 4) and compared several kinematic parameters (Table 1). Data were collected from two groups: 20 trials (5 each to left head, right head, left tail, and right tail) from six desb420 mutants and five wild-type animals, and 20 trials from six desb420 mutants and four wild-type siblings. The trials were analyzed via a computer program written to automatically extract several parameters for each frame (Liu and Fetcho, 1999
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Figure 4. desb420 mutant larvae exhibited primarily normal escape responses. A tap with a small polished glass probe elicited escapes. In this trial, the tap was delivered to the left side of the head (bottom left-hand corner). Images were captured at 1000 frames per second. Every third frame (msec) is shown, starting at the initiation of the response (frame 0). After the start of movement, peak turn angle is reached at 15 msec (15). For an example of a wild-type escape response, see Liu and Fetcho (1999
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Table 1. Escape response performance in wild-type and desb420 mutant larvae
Surprisingly, performance measurements that assess the function of Mauthner cells in the escape response were primarily unaffected in desb420 mutant larvae compared with wild-type larvae (Table 1). In particular, the peak angular velocity was unaffected (p > 0.05), suggesting that performance was not increased by the presence of extra Mauthner cells. The latency to respond was also not significantly different between mutant and wild-type larvae for both head- and tail-elicited responses (p > 0.05). Previous Mauthner cell lesion studies showed no effect on turn angle after killing the Mauthner cell and its hindbrain homologues (Liu and Fetcho, 1999
Mauthner axons in des mutants have fewer axon collaterals
Despite the presence of supernumerary Mauthner cells contributing to the circuit, the escape response in desb420 mutants was relatively unaffected. One explanation for this finding is that each Mauthner cell could be playing a correspondingly smaller role in mediating the escape behavior. Mauthner cells drive the escape response by synapsing directly onto contralateral interneurons and motoneurons in the spinal cord via axon collaterals (Fetcho and Faber, 1988
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Figure 5. The number of collaterals per Mauthner axon is dramatically decreased in des mutants. A, B, Four dpf wild-type (A), desb420 (B), and destp37 larvae were back-labeled from the caudal spinal cord with lysinated rhodamine dextran. The number of axon collaterals was quantitated over a three spinal cord hemisegment region in the midtrunk, and the number of Mauthner cells was counted under transmitted light (C). Arrowheads denote axon collaterals. Scale bar, 5 µm.
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Table 2. Axon collaterals in wild-type and des mutant larvae
These data suggest that there is a relationship between the number of axon collaterals and the number of Mauthner cells; that is, when more Mauthner cells are present, there are fewer axon collaterals per Mauthner axon. To examine the relationship between Mauthner cell number and the number of axon collaterals per Mauthner axon, we analyzed destp37 mutants (van Eeden et al., 1996
When there is a greater number of Mauthner cells, each Mauthner axon has fewer collaterals, suggesting that the Mauthner axons are dividing their synaptic targets in the spinal cord. If this were the case, we would expect Mauthner axons on the same side of the spinal cord to have nonoverlapping axon collaterals. To test this, two different fluorophore-conjugated dextrans were electroporated into two separate Mauthner cells on the same side of the hindbrain in desb420 mutants. The positions of the labeled collaterals from the two different Mauthner cells were analyzed under confocal microscopy. We found that of 61 axon collaterals analyzed, 93% did not overlap with collaterals from the other labeled axon (Fig. 6, Table 3). In the small number of cases in which we did see overlap (two pairs), the collaterals might be contacting the same postsynaptic targets; although, even in these cases, they could be contacting different but adjacent postsynaptic neurons. These data suggest that supernumerary Mauthner axons in mutant larvae are forming synapses with largely nonoverlapping populations of spinal neurons and dividing their target territory. Together, these data are consistent with the hypothesis that each Mauthner cell in des mutants exerts less of an effect on downstream spinal neurons, and participation in the escape response is distributed among the population of Mauthner cells, thus maintaining a primarily normal escape response.
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Figure 6. Collaterals from distinct Mauthner axons in desb420 mutants do not form in the same location. Two Mauthner cell bodies in desb420 mutants were electroporated with different fluorophores, and their axon collaterals were imaged at 6 dpf. One axon is shown in red (A), and the other is shown in green (B). The merged image (C) shows that the collaterals from the two axons do not form in the same location. Arrowheads denote collaterals. Scale bar, 10 µm
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Table 3. Mauthner axon collaterals from distinct axons in desb420 mutants rarely form in the same position
Discussion
The escape response in zebrafish is initiated by Mauthner cells, a single pair of large reticulospinal neurons. A mutation in the zebrafish gene des/notch1a results in a dramatic increase in the number of Mauthner cells without an equivalent increase in other neurons within the neural circuit that drives the escape response (Gray et al., 2001Mauthner cell and the escape response
Both experimental manipulations and genetic perturbations have been used to study the affect of cell loss on the escape-response circuit. Ablating Mauthner cells in wild-type animals causes a serious diminution of the tail-elicited escape response, whereas the head-elicited escape appears unchanged, suggesting that the Mauthner cell is the principal interneuron mediating the tail-elicited response (Liu and Fetcho, 1999Fish and premetamorphic amphibians have only a single, large, fast-conducting Mauthner cell that initiates the escape response. However, a similar response in mammals is primarily mediated by a population of 20-60 "giant neurons" in the caudal pontine-reticular formation in the brainstem (Lingenhohl and Friauf, 1992
Mauthner axon collaterals
Our data show that there is a relationship between the number of Mauthner cells and the number of collaterals per Mauthner axon. It remains to be determined how the number and distribution of Mauthner axon collaterals are regulated. It may be that a Mauthner cell is sensitive to the presence of other Mauthner cells. Whether this regulation occurs at the level of the Mauthner cell body or axon is unclear. Alternatively, target cells in the spinal cord may mediate regulation. It is possible that once a spinal neuron is innervated by a Mauthner axon, it is bypassed by other Mauthner axons. On the basis of our data, we would predict that individual Mauthner cells in des mutants would have decreased output caused by their decreased numbers of axon collaterals compared with wild types. One way to test this idea would be to eliminate Mauthner cells and examine performance changes. We tried to laser ablate all but one Mauthner cell in desb420 mutants to get the biggest possible behavioral effect. Unfortunately, the tight juxtaposition of the Mauthner cell bodies makes controlled removal of the cells using dye phototoxicity very difficult, rendering this experiment unfeasible. Therefore, our data are consistent with this hypothesis, although the difficulties with selective ablations precluded a direct assessment of the contribution of each of the cells to the behavior.Homozygous des mutants have other defects that could potentially effect the formation of Mauthner axon collaterals. For example, des mutants have mispatterned somites and defects in axon guidance (van Eeden et al., 1996
Our data show that all Mauthner cells in desb420 mutants are activated during an elicited escape response (Fig. 2). However, it is possible that different Mauthner cells in mutants contribute unequally to the response. For example, some Mauthner axons could have many collaterals and thus a stronger input onto spinal neurons, whereas other Mauthner axons could have fewer collaterals and less of an impact on spinal neurons. The totality of these responses would result in a normal escape response. However, the axon collateral data do not support this idea. Although there was variability in the number of axon collaterals counted, there was no clear subgrouping of axons having the wild-type number of collaterals and other axons having substantially fewer collaterals (Tables 2, 3). The one exception to this was an example in destp37 in which there were only two Mauthner cells, and one of them had 12 collaterals over the three spinal cord hemisegment distance (Table 2). This number of collaterals was the smallest number seen in wild-type larvae (range, 12-18 collaterals per 3 hemisegments) and raises the possibility that when only two Mauthner cells are present, the number of collaterals approximates what is seen in wild-type larvae, where there is only one Mauthner cell. However, as soon as there are three Mauthner cells present, the number of collaterals decreases significantly (range, 4-8 collaterals per 3 hemisegments). Thus, there appears to be an overall decrease in the axon collateral number on each axon rather than a large decrease in collaterals on some axons.
Evolution of the escape response
Analysis of des mutants may yield insight into the evolution of the escape response. As mentioned above, a startle response in mammals analogous to the fish escape response is mediated by a population of 20-60 neurons in the caudal pontine-reticular formation that contacts spinal interneurons and motoneurons (Lingenhohl and Friauf, 1992
Footnotes
Received May 1, 2003; revised July 3, 2003; accepted July 16, 2003.This work was supported by a postdoctoral fellowship from the Helen Hay Whitney Foundation (K.S.L.), National Institute of Neurological Disorders and Stroke Grant F31 NS11056-01A1 (M.G.), National Institutes of Health Grant NS26539 (J.R.F.), and National Science Foundation Grant IBN-9817076 (C.E.B.). We thank the support staff of our zebrafish facilities for maintaining fish lines, and Cecilia Moens (Fred Hutchinson Cancer Reserach Center, Seattle, WA) for helpful comments on this manuscript. The 3A10 monoclonal antibody, developed by Thomas M. Jessell and Jane Dodd (Columbia University, New York, NY), was obtained from the Developmental Studies Hybridoma Bank, developed under the auspices of the National Institute of Child Health and Human Development, and maintained by The University of Iowa Department of Biological Sciences.
Correspondence should be addressed to Christine E. Beattie, Department of Neuroscience, Center for Molecular Neurobiology, 115 Rightmire Hall, 1060 Carmack Road, Columbus, OH 43210. E-mail: beattie.24{at}osu.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/238159-08$15.00/0
* K.S.L. and M.G. contributed equally to this work.
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