Diversity in neuroblast number forming mushroom bodies of the higher dipterans (Insecta,Diptera, Brachycera Cyclorrhapha)

Neurogenesis in mushroom bodies is studied in 12 species of the higher dipterans. A significant difference in the number of neuroblasts forming mushroom bodies is found. In the majority of species studied, Kenyon cells are formed by four solitary neuroblasts. Among six calliphorid species, the number of neuroblasts increases up to 10–15 (mean 12.6) in each mushroom body in Calliphora vicina only. In young pupae of Muscina stabulans and M. livida, four polyneuroblastic prolipherative centers occur instead of solitary neuroblasts. These centers disintegrate later into numerous solitary neuroblasts. A hypothesis on the origin of the polyneuroblastic structure of mushroom bodies found in C. vicina and, earlier, in Musca domestica, is proposed.     

A subpopulation of mushroom body intrinsic neurons is generated by protocerebral neuroblasts in the tobacco hornworm moth, Manduca sexta (Sphingidae, Lepidoptera)

Subpopulations of Kenyon cells, the intrinsic neurons of the insect mushroom bodies, are typically sequentially generated by dedicated neuroblasts that begin proliferating during embryogenesis. When present, Class III Kenyon cells are thought to be the first born population of neurons by virtue of the location of their cell somata, farthest from the position of the mushroom body neuroblasts. In the adult tobacco hornworm moth Manduca sexta, the axons of Class III Kenyon cells form a separate Y tract and dorsal and ventral lobelet; surprisingly, these distinctive structures are absent from the larval Manduca mushroom bodies. BrdU labeling and immunohistochemical staining reveal that Class III Kenyon cells are in fact born in the mid-larval through adult stages. The peripheral position of their cell bodies is due to their genesis from two previously undescribed protocerebral neuroblasts distinct from the mushroom body neuroblasts that generate the other Kenyon cell types. These findings challenge the notion that all Kenyon cells are produced solely by the mushroom body neuroblasts, and may explain why Class III Kenyon cells are found sporadically across the insects, suggesting that when present, they may arise through de novo recruitment of neuroblasts outside of the mushroom bodies. In addition, lifelong neurogenesis by both the Class III neuroblasts and the mushroom body neuroblasts was observed, raising the possibility that adult neurogenesis may play a role in mushroom body function in Manduca.     

How many neuroblasts build mushroom bodies in <Emphasis Type="Italic">Lucilia caesar</Emphasis> L. and <Emphasis Type="Italic">Musca domestica</Emphasis> L. (Diptera,Brachycera Cyclorrhapha)?

The green-bottle fly Lucilia caesar and the housefly Musca domestica differ greatly in the number of neuroblasts producing mushroom bodies. Four neuroblasts were found in each mushroom body of Lucilia pupae, and its calyx has a quadruple structure. In the housefly, the number of mushroom body neuroblasts rises up 20 in each brain hemisphere. This leads to a more complicated calyx structure. The neuroblast number observed in Lucilia and Musca is compared with that found in other Diptera.     

中华蜜蜂蕈形体的发育

中华蜜蜂(Apis cerana cerana)的脑由前脑、中脑和后脑三部分构成,蕈形体位于前脑的背侧,是其重要的学习及其他复杂行为的整合中心。通过对中华蜜蜂工蜂的幼虫、蛹及成虫的蕈形体形态发育的观察研究,发现中华蜜蜂的蕈形体包含约1000个成神经细胞,它们最终形成了蕈形体的所有Kenyon细胞。这些成神经细胞来自于在新孵化的幼虫脑中已存在的四丛成神经细胞,每一丛细胞的数量不多于45个。蕈形体柄区的出现约在3龄幼虫,而α叶和β叶在5龄幼虫已可明显辨认。冠区出现较晚,大约在蛹期的第二天以后。由于社会性昆虫复杂的学习、记忆和认知需求,其蕈形体的体积和复杂程度都优于其他昆虫。     

Proliferation pattern of postembryonic neuroblasts in the brain of Drosophila melanogaster.

The spatio-temporal proliferation pattern of postembryonic neuroblasts in the central brain region of the supra-esophageal ganglion of Drosophila melanogaster was studied by labeling DNA replicating cells with 5-bromo-2'-deoxyuridine (BrdU). There are five proliferating neuroblasts per hemisphere in larvae just after hatching: one in the ventro-lateral, and the other four in the postero-dorsal region of the brain. Dividing neuroblasts increase during the late first-late second instar larval stages, reaching a plateau of about 85 neuroblasts per hemisphere. Most neuroblasts cease dividing 20-30 hr after puparium formation (APF), while only four in the postero-dorsal region continue making progenies until 85-90 hr APF. The four distinct neuroblasts proliferating in the early larval and late pupal stages are identical; they lie in the cortex above the calyces of the mushroom bodies (corpora pedunculata), proliferating over a period twice as long as that for the other neuroblasts. Their daughter neurons project into the mushroom body neuropile, and hence are likely to be the Kenyon cells. The cell-cycle period of the four neuroblasts (named mushroom body neuroblasts: MBNbs) is rather constant (1.1-1.5 hr) during the mid larval-early pupal stages and is longer before and after that. The total number of the MBNb progenies made throughout the embryonic and postembryonic development was estimated to be 800-1200 per hemisphere.     

Mitogenic effects of 20-hydroxyecdysone on neurogenesis in adult mushroom bodies of the cockroach, Diploptera punctata

The purpose of this study was to examine the mitogenic effects of 20-hydroxyecdysone on neurogenesis in mushroom bodies of the adult cockroach, Diploptera punctata. The occurrence of neurogenesis was studied immunocytochemically after in vivo labeling with 5-bromo-2'-deoxyuridine (BrdU). The number of BrdU-labeled cells in the mushroom bodies was high shortly after adult ecdysis, then gradually decreased, and proliferation ceased on day 8. 20-Hydroxyecdysone injection during the early adult stages significantly delayed the decrease in mitotic activity. Moreover, 20-hydroxyecdysone injection during the late stage stimulated quiescent mushroom body neuroblasts to initiate their mitotic activity in a dose-dependent manner. These results indicated that the mushroom body neuroblasts of this insect become quiescent in the maturing central nervous system, but retain the capacity for proliferation if exposed to appropriate environmental signals. We conclude that 20-hydroxyecdysone has a mitogenic effect on neurogenesis in mushroom bodies of this insect.     

Mcm3 replicative helicase mutation impairs neuroblast proliferation and memory in Drosophila

In the developing Drosophila brain, a small number of neural progenitor cells (neuroblasts) generate in a co‐ordinated manner a high variety of neuronal cells by integration of temporal, spatial and cell‐intrinsic information. In this study, we performed the molecular and phenotypic characterization of a structural brain mutant called small mushroom bodies (smu), which was isolated in a screen for mutants with altered brain structure. Focusing on the mushroom body neuroblast lineages we show that failure of neuroblasts to generate the normal number of mushroom body neurons (Kenyon cells) is the major cause of the smu phenotype. In particular, the premature loss of mushroom body neuroblasts caused a pronounced effect on the number of late‐born Kenyon cells. Neuroblasts showed no obvious defects in processes controlling asymmetric cell division, but generated less ganglion mother cells. Cloning of smu uncovered a single amino acid substitution in an evolutionarily conserved protein interaction domain of the Minichromosome maintenance 3 (Mcm3) protein. Mcm3 is part of the multimeric Cdc45/Mcm/GINS (CMG) complex, which functions as a helicase during DNA replication. We propose that at least in the case of mushroom body neuroblasts, timely replication is not only required for continuous proliferation but also for their survival. The absence of Kenyon cells in smu reduced learning and early phases of conditioned olfactory memory. Corresponding to the absence of late‐born Kenyon cells projecting to α′/β′ and α/β lobes, smu is profoundly defective in later phases of persistent memory.     

General structure of the mushroom body calyx in brachycera orthorrhapha flies (Diptera)

The mushroom body calyx in Brachycera Orthorrhapha flies is extremely diverse in the degree of development. In general, the calyx has the anterior, posterior, and dorsal lobes, as well as “sleeves” of glomerular neuropil surrounding Kenyon cell fibers. The anterior lobe of the calyx is found in all species studied. The most complex structure of the calyx is characteristic of the families Empididae and especially Bombyliidae, in which it has all the parts listed above. Brachycera Orthorrhapha flies have three fiber bundles of Kenyon cells, in contrast to four bundles in Drosophila. It is assumed that each mushroom body in Brachycera Orthorrhapha flies is formed by descendants of three single neuroblasts.     

Mitogenic effects of 20‐hydroxyecdysone on neurogenesis in adult mushroom bodies of the cockroach,Diploptera punctata

The purpose of this study was to examine the mitogenic effects of 20‐hydroxyecdysone on neurogenesis in mushroom bodies of the adult cockroach, Diploptera punctata. The occurrence of neurogenesis was studied immunocytochemically after in vivo labeling with 5‐bromo‐2′‐deoxyuridine (BrdU). The number of BrdU‐labeled cells in the mushroom bodies was high shortly after adult ecdysis, then gradually decreased, and proliferation ceased on day 8. 20‐Hydroxyecdysone injection during the early adult stages significantly delayed the decrease in mitotic activity. Moreover, 20‐hydroxyecdysone injection during the late stage stimulated quiescent mushroom body neuroblasts to initiate their mitotic activity in a dose‐dependent manner. These results indicated that the mushroom body neuroblasts of this insect become quiescent in the maturing central nervous system, but retain the capacity for proliferation if exposed to appropriate environmental signals. We conclude that 20‐hydroxyecdysone has a mitogenic effect on neurogenesis in mushroom bodies of this insect. © 1999 John Wiley & Sons, Inc. J Neurobiol 39: 264–274, 1999     

Early development of the Drosophila mushroom bodies, brain centres for associative learning and memory

We have studied the formation of Drosophila mushroom bodies using enhancer detector techniques to visualize specific components of these complex intrinsic brain structures. During embryogenesis, neuronal proliferation begins in four mushroom body neuroblasts and the major axonal pathways of the mushroom bodies are pioneered. During larval development, neuronal proliferation continues and further axonal projections in the pedunculus and lobes are formed in a highly structured manner characterized by spatial heterogeneity of reporter gene expression. Enhancer detector analysis identifies many genomic locations that are specifically activated in mushroom body intrinsic neurons (Kenyon cells) during the transition from embryonic to postembryonic development and during metamorphosis.     

Not all dytiscidae have poorly developed mushroom bodies: The enigma of Cybister lateralimarginalis

The majority of diving beetles studied has completely differentiated but poorly developed mushroom bodies. The Kenyon cells are not numerous, the calyces are small, and the pedunculi and lobes have a simple structure. New Kenyon cells are produced by few solitary neuroblasts. Cybister lateralimarginalis makes an amazing exception. Its mushroom bodies are strongly developed and comprise numerous Kenyon cells, large calyces, and a peduncular apparatus of a complicated structure. The Kenyon cells are produced in polyneuroblast proliferative centers. The grounds of such strong development of the mushroom body in Cybister remain unknown.     

Metamorphosis and adult development of the mushroom bodies of the red flour beetle, Tribolium castaneum

The insect mushroom bodies play important roles in a number of higher processing functions such as sensory integration, higher level olfactory processing, and spatial and associative learning and memory. These functions have been established through studies in a handful of tractable model systems, of which only the fruit fly Drosophila melanogaster has been readily amenable to genetic manipulations. The red flour beetle Tribolium castaneum has a sequenced genome and has been subject to the development of molecular tools for the ready manipulation of gene expression; however, little is known about the development and organization of the mushroom bodies of this insect. The present account bridges this gap by demonstrating that the organization of the Tribolium mushroom bodies is strikingly like that of the fruit fly, with the significant exception that the timeline of neurogenesis is shifted so that the last population of Kenyon cells is born entirely after adult eclosion. Tribolium Kenyon cells are generated by two large neuroblasts per hemisphere and segregate into an early-born delta lobe subpopulation followed by clear homologs of the Drosophila gamma, alpha'/beta' and alpha/beta lobe subpopulations, with the larval-born cohorts undergoing dendritic reorganization during metamorphosis. BrdU labeling and immunohistochemical staining also reveal that a proportion of individual Tribolium have variable numbers of mushroom body neuroblasts. If heritable, this variation represents a unique opportunity for further studies of the genetic control of brain region size through the control of neuroblast number and cell cycle dynamics.     

Fate of neuroblast progeny during postembryonic development of mushroom bodies in the house cricket,Acheta domesticus

Mushroom bodies represent the main sensory integrative center of the insect brain and probably play a major role in the adaptation of behavioral responses to the environment. Taking into account the continuous neurogenesis of cricket mushroom bodies, we investigated ontogenesis of this brain structure. Using BrdU labeling, we examined the fate of neuroblast progeny during the postembryonic development. Preimaginal Kenyon cells survived throughout larval and imaginal moults and persisted during adulthood. Our results indicate that the location of labelled Kenyon cells in the cortex of the adult cricket mainly depends upon the period when they were produced during development. The present data demonstrate that cricket mushroom bodies grow from the inside out and that, at any developmental stage, the center of the cortex contains the youngest Kenyon cells. This study also allowed us to observe the occurrence of quiescent neuroblasts. Kenyon cell death during postembryonic and adult life seems to be reduced. Although preimaginal Kenyon cells largely contribute to adult mushroom body structure, a permanent remodeling of the mushroom body occurs throughout the whole insect life due to the persistence of neurogenesis in the house cricket. Further studies are needed to understand the functional significance of these findings.     

Longicorn beetles (Coleoptera: Cerambycidae) differ considerably in the degree of their mushroom body development

A duality in the general structure of the mushroom body in longicorn beetles is confirmed. This duality is associated with the fact that they are formed by two solitary neuroblasts or two neuroblast clusters on each side of the brain and are manifested as a bipartite structure of both the calyx, which is the main sensory input, and the peduncular apparatus. Within the studied longicorn beetles, modifications in the general structure of mushroom bodies have been found; these modifications are caused by two oppositely directed morphogenetic processes, namely, the concentration of structures and their compartmentalization. The concentration leads to disappearance of the bipartite structure of the peduncular apparatus, whereas compartmentalization leads to a secondary subdivision of these structures into anatomically distinct subsections. This process is most pronounced in the peduncle and lobes. The mushroom bodies are best developed and differentiated in the members of the subfamily Lamiinae.     

Developmental organization of the mushroom bodies of Thermobia domestica (Zygentoma, Lepismatidae): insights into mushroom body evolution from a basal insect

The mushroom bodies of the insect brain are sensory integration centers best studied for their role in learning and memory. Studies of mushroom body structure and development in neopteran insects have revealed conserved morphogenetic mechanisms. The sequential production of morphologically distinct intrinsic neuron (Kenyon cell) subpopulations by mushroom body neuroblasts and the integration of newborn neurons via a discrete ingrowth tract results in an age-based organization of modular subunits in the primary output neuropil of the mushroom bodies, the lobes. To determine whether these may represent ancestral characteristics, the present account assesses mushroom body organization and development in the basal wingless insect Thermobia domestica. In this insect, a single calyx supplied by the progeny of two neuroblast clusters, and three perpendicularly oriented lobes are readily identifiable. The lobes are subdivided into 15 globular subdivisions (Trauben). Lifelong neurogenesis is observed, with axons of newborn Kenyon cells entering the lobes via an ingrowth core. The Trauben do not appear progressively during development, indicating that they do not represent the ramifications of sequentially produced subpopulations of Kenyon cells. Instead, a single Kenyon cell population produces highly branched axons that supply all lobe subdivisions. This suggests that although the ground plan for neopteran mushroom bodies existed in early insects, the organization of modular subunits composed of separate Kenyon cell subpopulations is a later innovation. Similarities between the calyx of Thermobia and the highly derived fruit fly Drosophila melanogaster also suggest a correlation between calyx morphology and Kenyon cell number.     

Comparative histology of mushroom bodies in carnivorous beetles of the suborder polyphaga (Insecta, Coleoptera)

Mushroom bodies in beetles of the families Histeridae, Staphylinidae, Cantharidae, Trogossitidae, Peltidae, Cleridae, Malachiidae, and Coccinellidae are shown to be rather poorly developed. The calyx region of the mushroom bodies in these beetles never forms two separate cups, and the peduncular apparatus includes a unified shaft almost over its entire length. Only the pedunculus contains two separate shafts in a few cases. Two proliferative centers consisting of one to three neuroblasts are often found in each Kenyon cell group. The shift from carnivorous to feeding on pollen or leaves, which has taken place in some taxa, does not visibly affect the degree of mushroom body development.     

Influence of environmental stimulation on neurogenesis in the adult insect brain

Mushroom bodies are the main integrative structures of insect brain. They receive sensory information from the eyes, the palps, and the antennae. In the house cricket, Acheta domesticus, a cluster of mushroom body neuroblasts keeps producing new interneurons during an insect's life span. The aim of the present work is to study the impact of environmental stimuli on mushroom body neurogenesis during adulthood. Crickets were reared either in an enriched environment, where they received complex environmental and congeneric stimulations or isolated in small cages and deprived of most visual, auditory, and olfactory stimuli. They then were injected with a S-phase marker, 5-bromo, 2'-deoxyuridine (BrdU) and sacrificed at different periods of their life. Neurogenesis and cell survival were estimated by counting the number of BrdU-labeled cells in the mushroom bodies. Environmentally enriched crickets were found to have an increased number of newborn cells in their mushroom bodies compared with crickets housed in cages with an impoverished environment. This effect of external factors on neurogenesis seems to be limited to the beginning of imaginal life. Furthermore, no cell loss could be detected among the newborn neurons in either environmental situation, suggesting that cell survival was not affected by the quality of the environment. Considering vertebrate studies which showed that enriched environment increases hippocampal cell survival and improves animal performances in spatial learning tests, we suggest that the increased number of interneurons produced in an integrative brain structure after exposure to enriched environment could contribute to adaptive behavioral performances in adult insects.     

Early development of the Drosophila mushroom body: the roles of eyeless and dachshund

The mushroom body (MB) is a uniquely identifiable brain structure present in most arthropods. Functional studies have established its role in learning and memory. Here we describe the early embryonic origin of the four neuroblasts that give rise to the mushroom body and follow its morphogenesis through later embryonic stages. In the late embryo, axons of MB neurons lay down a characteristic pattern of pathways. eyeless (ey) and dachshund (dac) are expressed in the progenitor cells and neurons of the MB in the embryo and larva. In the larval brains of the hypomorphic ey(R) strain, we find that beside an overall reduction of MB neurons, one MB pathway, the medial lobe, is malformed or missing. Overexpression of eyeless in MBs under the control of an MB-specific promoter results in a converse type of axon pathway abnormality, i.e. malformation or loss of the dorsal lobe. In contrast, loss of dachshund results in deformation of the dorsal lobe, whereas no lobe abnormalities can be detected following dachshund overexpression. These results indicate that ey and dachshund may have a role in axon pathway selection during embryogenesis.