神经发育中的一些新发现的轴突导向因子

神经发育过程中,存在一些引导轴突向特定靶区生长的导向因子。这些因子以浓度梯度型式作用,或者与细胞膜相连起信号转导作用。主要介绍近来发现几类新的轴突导向因子家族：ｎｅｔｒｉｎ家族、ｓｅｍａｐｈｏｒｉｎ家族、ｃｏｎｎｅｃｔｉｈ家族、Ｅｐｈ受体家族及其配体家族,以及其它的轴突导向因子。     

轴突导向因子参与神经病理痛的研究进展

轴突导向因子协同引导轴突延伸，准确地进行轴突的投射。神经系统损害发生后，这些因子及其各自受体相互作用，通过激活磷酸激酶，影响突触可塑性从而诱发和维持神经病理痛。     

Eph-ephrin与突触可塑性

Eph受体酪氨酸激酶及其配体ephrin广泛参与神经系统的发育,如轴突导向、细胞迁移、体节形成和血管生成。最近研究显示的Ephephrin在突触的定位提示其与突触可塑性有关。Ephephrin对成年神经系统的可塑性、学习和记忆,以及神经损伤后的再生可能具有重要的调节作用。     

损伤相关模式分子与慢性疾病

损伤相关模式分子是组织或细胞受到损伤、缺氧、应激等因素刺激后释放到细胞间隙或血液循环中的一类物质,可通过Toll样受体、RIG-1样受体或NOD样受体等模式识别受体,诱导自身免疫或免疫耐受,在关节炎、动脉粥样硬化、肿瘤、系统性红斑狼疮等疾病发生和发展过程中发挥重要作用.现已发现的损伤相关分子模式分子包括细胞内蛋白分子、非蛋白嘌呤类分子及其降解产物、细胞外基质降解产物和无引导序列免疫细胞因子如IL-1 和IL-18等.损伤相关模式分子的发现及其作用机制的阐明,将有助于阐明多种慢性炎症疾病的病理机制,为这些疾病的诊断和防治提供新的思路.本文综述了主要的损伤相关模式分子的概念、释放方式,及其与模式识别受体相互作用引起炎症反应和参与多种慢性疾病过程的机制.     

ROBO4 与缺血性脑血管病相关的研究进展

Roundabout(Robo)蛋白是神经轴突导向分子家族Slit蛋白的单次跨膜受体,属于一种神经细胞粘附分子。Robo蛋白在神经系统已被确认具有重要轴突导向功能。近年来研究发现,血管新生的内皮细胞表面只特异性地表达Robo4,且Robo4对内皮细胞迁移、病理性血管生成和血管完整性都具有调节作用。缺血性脑血管病是人类致残甚至死亡的主要疾病之一,由于短暂或持续的脑血流减少而造成脑细胞损伤,因此,恢复脑血流、促进血管再生对脑功能恢复至关重要。Robo4对血管方面的作用为我们进一步研究及了解其在血管生成中的机制提供重要依据,也为缺血性脑血管病的治疗提供新的发展方向。     

Slit/Robo信号在血管新生中的功能研究

分泌型糖蛋白Slit及其受体Roundabout(Robo)最初是作为一类重要的发育中神经元轴突导向分子而被发现的。目前为止对Slit/Robo信号对神经系统发育过程中轴突吸引或排斥的导向功能研究比较多,而对在发育中生长方式与其非常相似的血管发生过程中研究比较少。现有研究提示两者在发育过程中可能存在共同的信号调控机制,是Slit/Robo信号通路在血管新生中充当着重要的角色。该文就Slit/Robo信号对血管内皮细胞迁移的调节、对血管新生的作用及其可能介导的信号通路进行综述,以期进一步推动Slit/Robo信号通路在血管发生中的研究。     

神经轴突导向分子Robo的功能及其分子作用机制研究进展(英文)

神经轴突导向分子Robo是进化上高度保守的跨膜蛋白。Robo及其配体Slit对神经轴突导向、神经细胞迁移、肿瘤转移、血管生成、肺脏、肾脏、心脏的形态发生以及卵巢、性腺的发育等多项生命活动具有调节作用。Robo功能的实现主要通过其Ig1结构域与其配体Slit的LRR-2结构域结合,同时也通过与多种信号分子如硫酸肝素蛋白多糖(heparan sulfate proteoglycans,HSPGs)、GTP酶激活蛋白(GTPase-activating proteins,GAPs)、酪氨酸激酶Abelson等结合发挥作用。robo基因的表达受到Hox、Midline、Nkx2.9等转录因子的调节,另外,转录后水平上的选择性剪接和转录产物的转运等调控也影响Robo的功能。本文对Robo蛋白的结构与功能以及分子作用机制等研究进展进行了综述,以期为神经发育研究和神经系统疾病与癌症防治提供新思路。     

无脊椎动物免疫分子多态性

 一般认为,非特异性免疫分子由于胚系基因种类有限而不具备多态性.但近年来人们发现,脊椎动物γ/δ T 细胞受体、B1细胞受体、某些固有免疫成分,以及无脊椎动物的某些免疫球蛋白超家族（immunoglobulin superfamily,IgSF）分子、抗菌肽和模式识别受体（pattern recognition receptors,PRR）等同样具有较高程度的多态性.与特异性免疫分子相似,其多态性形成机制主要为基因组水平的基因重排、单核苷酸多态性、DNA 突变和 mRNA 水平的外显子可变剪接.该多态性的出现可能是无脊椎动物的一种适应性进化,其应为低等生物特异性识别和防御不同病原微生物感染的分子基础. 本文就无脊椎动物免疫分子多态性的最新研究进展及其可能的形成机制与意义进行概述.     

无脊椎动物免疫分子的多态性

一般认为,非特异性免疫分子由于胚系基因种类有限而不具备多态性.但近年来人们发现,脊椎动物γ/δT细胞受体、B1细胞受体、某些固有免疫成分,以及无脊椎动物的某些免疫球蛋白超家族(immunoglobulin superfamily,IgSF)分子、抗菌肽和模式识别受体(pattern recognition receptors,PRR)等同样具有较高程度的多态性.与特异性免疫分子相似,其多态性形成机制主要为基因组水平的基因重排、单核苷酸多态性、DNA突变和mRNA水平的外显子可变剪接.该多态性的出现可能是无脊椎动物的一种适应性进化,其应为低等生物特异性识别和防御不同病原微生物感染的分子基础.本文就无脊椎动物免疫分子多态性的最新研究进展及其可能的形成机制与意义进行概述.     

烟碱型乙酰胆碱受体及其神经保护作用

新近研究证实,神经元烟碱型乙酰胆碱受体(nAChR)激动后可起到一定的神经保护作用.目前,一些作用于烟碱受体的激动剂已被作为治疗神经退行性疾病如阿尔茨海默病(AD)和帕金森病(PD)的候选药物,但是关于烟碱受体激动后如何发挥神经保护作用及其潜在的分子机制还不清楚,其中有与Ca2+相关的信号转导假说以及神经营养因子等假说.本文就烟碱型乙酰胆碱受体及其神经保护作用的研究进展予以综述.     

Effect of vesicle traps on traffic jam formation in fast axonal transport

The purpose of this paper is to develop a model for simulation of the formation of organelle traps in fast axonal transport. Such traps may form in the regions of microtubule polar mismatching. Depending on the orientation of microtubules pointing toward the trap region, these traps can accumulate either plus-end or minus-end oriented vesicles. The model predicts that the maximum concentrations of organelles occur at the boundaries of the trap regions; the overall concentration of organelles in the axon with traps is greatly increased compared to that in a healthy axon, which is expected to contribute to mechanical damages of the axon. The organelle traps induce hindrance to organelle transport down the axon; the total organelle flux down the axon with traps is found to be significantly reduced compared to that in a healthy axon.     

Transcriptional regulators that differentially control dendrite and axon development

Neurons are the basic units of connectivity in the nervous system.As a signature feature,neurons form polarized structures:dendrites and axons,which integrate either sensory stimuli or inputs from upst...     

神经退变和再生过程中郎氏结构筑的变化

将夹伤的大鼠坐骨神经分离成单根纤维,在光镜、扫描和透射电镜下观察伤后９８天内郎氏结的构筑变化。发现损伤使细胞器的轴浆转运阻断,积累的退变细胞器使结区的轴突外凸,郎氏结构构筑变形,髓鞘板层失序,轴膜崩解,积累的细胞器逸出,并看到仅残存的郎氏结近心端构筑、由近心端的母体神经和远心端的再生神经共同构筑的新生郎氏结,以及新生郎氏结构的发育过程等特征性图象。再生轴突中转运的微管等细胞器和施旺细胞中富含的线粒     

Effect of the degree of polar mismatching on traffic jam formation in fast axonal transport

This paper simulates an axon with a region of reversed microtubule (MT) polarity, and investigates how the degree of polar mismatching in this region affects the formation of organelle traps in the axon. The model is based on modified Smith–Simmons equations governing molecular-motor-assisted transport in neurons. It is established that the structure that develops as a result of a region with disoriented MTs consists of two organelle traps, the trap to the left of this region accumulates plus-end-oriented organelles and the trap to the right of this region accumulates minus-end-oriented organelles. The presence of such a structure is shown to inhibit the transport of organelles down the axon. The degree by which the transport of organelles is inhibited depends on the degree of polar mismatching of MTs in the region between MT traps. Four cases with a different degree of polar mismatching are investigated.     

Glia engulf degenerating axons during developmental axon pruning

Developmental axon pruning is widely used in constructing the nervous system. Accordingly, diverse mechanisms are likely employed for various forms of axon pruning. In the Drosophila mushroom bodies (MB), gamma neurons initially extend axon branches into both the dorsal and medial MB axon lobes in larvae. Through a well-orchestrated set of developmental events during metamorphosis, axon branches to both lobes degenerate prior to the formation of adult connections. Here, we analyze ultrastructural changes underlying axon pruning by using a genetically encoded electron microscopic (EM) marker to selectively label gamma neurons. By inhibiting axon pruning in combination with the use of this EM marker, we demonstrate a causal link between observed cellular events and axon pruning. These events include changes in axon ultrastructure, synaptic degeneration, and engulfment of degenerating axon fragments by glia for their subsequent breakdown via the endosomal-lysosomal pathway. Interestingly, glia selectively invade MB axon lobes at the onset of metamorphosis; this increase in cell number is independent of axon fragmentation. Our study reveals a key role for glia in the removal of axon fragments during developmental axon pruning.     

Drosophila multiplexin (Dmp) modulates motor axon pathfinding accuracy

Multiplexins are multidomain collagens typically composed of an N‐terminal thrombospondin‐related domain, an interrupted triple helix and a C‐terminal endostatin domain. They feature a clear regulatory function in the development of different tissues, which is chiefly conveyed by the endostatin domain. This domain can be found in proteolytically released monomeric and trimeric versions, and their diverse and opposed effects on the migratory behavior of epithelial and endothelial cell types have been demonstrated in cell culture experiments. The only Drosophila multiplexin displays specific features of both vertebrate multiplexins, collagens XV and XVIII. We characterized the Drosophila multiplexin (dmp) gene and found that three main isoforms are expressed from it, one of which is the monomeric endostatin version. Generation of dmp deletion alleles revealed that Dmp plays a role in motor axon pathfinding, as the mutants exhibit ventral bypass defects of the intersegmental nerve b (ISNb) similar to other motor axon guidance mutants. Transgenic overexpression of monomeric endostatin as well as of full‐length Dmp, but not trimeric endostatin, were able to rescue these defects. In contrast, trimeric endostatin increased axon pathfinding accuracy in wild type background. We conclude that Dmp plays a modulating role in motor axon pathfinding and may be part of a buffering system that functions to avoid innervation errors.     

Effects of neuropathic and non-neuropathic isomers of tricresyl phosphate and their microsomal activation on the production of axon-like processes by differentiating mouse N2a neuroblastoma cells

The aim of this work was to investigate the sublethal neuropathic effects of tricresyl phosphate (TCP: mixed isomers), triorthocresyl phosphate (TO:CP) and triparacresyl phosphate (TP:CP) on differentiating mouse N2a neuroblastoma cells. This was achieved by a combination of measurements of cell viability, axon outgrowth and the levels of cytoskeletal proteins detectable on western blots of extracts from cells induced to differentiate in the presence and absence of the compounds. In a time-course experiment TCP inhibited the outgrowth of axon-like processes following exposure times of 24 h or longer. Dose-response experiments indicated that TCP and TO:CP exhibited similar sustained levels of toxicity following both 24 and 48 h exposure, with no significant difference between their respective IC(50) values. By contrast, TP:CP demonstrated a transient effect on the outgrowth of axon-like processes, which was detectable after 24 but not 48 h of exposure. Isomer-specific patterns of toxicity were also evident at earlier time-points, with only the ortho isomer showing significant levels of inhibition of axon outgrowth following 4-8 h exposure. Probing of western blots with antibodies against cytoskeletal proteins indicated that the inhibition of axon outgrowth by these compounds was associated with a sustained reduction in the levels of phosphorylated neurofilament heavy chain. The inhibitory effect on axon outgrowth of TO:CP but not TP:CP was enhanced in the presence of a microsomal activation system. Since TO:CP is the most neuropathic of the isomers of TCP in vivo, differentiating N2a cells provide a useful cellular system for mechanistic studies of the neurodegenerative effects of this organophosphate.     

Modelling transport of layered double hydroxide nanoparticles in axons and dendrites of cortical neurons

This paper develops a model of nanoparticle transport in neurons. It is assumed that nanoparticles are transported inside endocytic vesicles by a combined effect of dynein-driven transport and diffusion. It is further assumed that in axons nanoparticles are internalised only at axon terminals, whereas in dendrites nanoparticles can enter through the entire plasma membrane. This causes differences in transport of nanoparticles in axons and dendrites; these differences are investigated in this paper. Another difference is microtubule (MT) orientation in axons and dendrites; in axons, all MTs have their plus-ends oriented towards the axon terminal; in a proximal region of a dendrite, MTs have mixed orientation, whereas in a distal dendritic region the MT orientation is similar to that in an axon. It is shown that if molecular-motor-driven transport were powered by dynein alone, such MT orientation in a dendrite would result in a region of nanoparticle accumulation located at the border between the proximal and distal dendritic regions.     

Axon regeneration across the site of injury in the optic nerve of the newt Triturus pyrrhogaster

Summary The process by which axons regenerate following a freeze injury to the optic nerve of the newt was analyzed by light and electron microscopy. Freezing destroys cellular constituents in a one millimeter segment of the nerve, leaving intact the basal lamina and the blood supply to the eye. No axons are seen at the site of injury one to seven days post lesion. This contrasts with the persistence of normal-appearing but severed unmyelinated axons within the cranial stump which thus give a false appearance of early regeneration. The first axon sprouts traverse the lesion and enter the cranial stump by ten days. The number of regenerating axons increases rapidly thereafter with no signs of random growth at the site of injury. These axon sprouts tend to be somewhat larger than normal unmyelinated axons and contain dense core vesicles and abnormal organelles similar to those in growing axons in tissue culture. The persisting basal lamina inside the optic sheath appears to provide continuity across the site of injury, to orient axon sprouts, and to favor an orderly process of axon regeneration without neuroma formation.The authors wish to express their gratitude to Barbara Heindel and Jill Jones for extremely helpful technical assistance. This work was supported by grants NS 10864 and NS 05666 from the U.S. Public Health Service and by the Medical Research Service of the Veterans Administration     

Rac proteins and the control of axon development

Rac GTPases and their effectors control cellular morphogenesis in a wide range of developmental contexts by regulating the structure and dynamics of the actin cytoskeleton. Although much is known about the biochemistry of Racs and Rac regulators, less is known about how Racs control cellular morphogenesis, including axon development, in vivo. Recent loss-of-function genetic studies using model organisms have shown that Racs and their effectors are required for multiple aspects of axon development, including axon outgrowth, axon guidance and axon branching. Interestingly, these studies have also revealed that Rac activity is required to prune spurious axons and branches. Analyses of Racs and their upstream and downstream effectors suggest that Rac signaling is complex. Different neurons utilize distinct combinations of upstream Rac regulators during axon development, possibly reflecting responses to different axon path-finding signals, and Racs use distinct downstream effectors to mediate different aspects of axon development, possibly reflecting differential regulation of the lamellipodial and filopodial growth-cone actin-cytoskeleton domains underlying axon developmental events.