Kinases regulating Golgi apparatus structure and function

Protein kinases control Golgi function in both mitotic and interphase cells. In mitosis, phosphorylation of structural proteins by Cdk1 (cyclin-dependent kinase 1)-cyclin B, Polo-like and mitogen-activated protein kinases underlie changes in Golgi reorganization during cell division. While in interphase, signalling pathways that are associated with the Golgi control secretory function through a variety of mechanisms. Some of these, notably those involving protein kinase D and Ste20 family kinases, are also relevant for the establishment and maintenance of cell polarization and migration.     

Camillo Golgi and the discovery of the Golgi apparatus

 Camillo Golgi (1843–1926) was born at Corteno, near Brescia, in northern Italy. After graduating in Medicine at the ancient University of Pavia, the former seat of great scientists and naturalists, Golgi continued a long-standing Italian tradition by studying the histology of the nervous system. While working as a modest physician at Abbiategrasso, a small town near Pavia, he developed a silver–osmium technique, the ”reazione nera” (black reaction), for which he was awarded the Nobel Prize in 1906. In the late 1890’s, 25 years after the publication of his black reaction and while Professor of General Pathology in Pavia, Golgi noticed a fine internal network in only partially silver-osmium-blackened Purkinje cells. Following confirmation by his assistant Emilio Veratti, Golgi published the discovery, called the ”apparato reticolare interno”, in the Bollettino della Società medico-chirurgica di Pavia in 1898, which is now considered the birthday of the ”Golgi apparatus”. The discovery of the Golgi apparatus can be added to the long list of accidental discoveries. The man after whom it is named was not a cytologist engaged in studying the inner structure of the cell, but a pathologist searching to prove a neuroanatomical theory. Accepted: 24 October 1997     

Positioning the Golgi apparatus

Ríos et al. (2004) report in this issue that the Golgi protein GMAP-210 is sufficient to confer pericentrosomal positioning and recruits gamma-tubulin and associated microtubule-nucleating ring complex proteins to Golgi membranes. The results raise the possibility that short microtubules emanate from the Golgi to mediate its organization and positioning.     

Subcompartmentalizing the Golgi apparatus

The subcompartmentalized structure of the Golgi apparatus contributes to efficient glycosylation in the secretory pathway. Subcompartmentalization driven by maturation relies primarily on constant and accurate vesicle-mediated local recycling of Golgi residents. The precision of this vesicle transport is dependent on the interplay between the key factors that mediate vesicle budding and fusion--the coat proteins and the SNARE fusion machinery. These alone, however, may not be sufficient to ensure establishment of compartments de novo, and additional regulatory mechanisms operate to modify their activity.     

Organization of the Golgi apparatus

Investigators are revisiting basic concepts of the structure-function relationships of the Golgi apparatus. A key issue is the properties of the transport carriers that operate within the secretory pathway. Golgi morphology and dynamics differ between species but data from various model systems are pointing toward an integrated view of Golgi organization.     

Calcium in the Golgi apparatus

The secretory-pathway Ca2+-ATPases (SPCAs) represent a recently recognized family of phosphorylation-type ATPases that supply the lumen of the Golgi apparatus with Ca2+ and Mn2+ needed for the normal functioning of this structure. Mutations of the human SPCA1 gene (ATP2C1) cause Hailey-Hailey disease, an autosomal dominant skin disorder in which keratinocytes in the suprabasal layer of the epidermis detach. We will first review the physiology of the SPCAs and then discuss how mutated SPCA1 proteins can lead to an epidermal disorder.     

Structure of Golgi apparatus

Summary Golgi apparatus (GA) of eukaryotic cells consist of one or more stacks of flattened saccules (cisternae) and an array of fenestrae and tubules continuous with the peripheral edges of the saccules. Golgi apparatus also are characterized by zones of exclusion that surround each stack and by an assortment of vesicles (or vesicle buds) associated with both the stacks and the peripheral tubules of the stack cisternae. Each stack (sometimes referred to as Golgi apparatus, Golgi complex, or dictyosome) is structurally and functionally polarized, reflecting its role as an intermediate between the endoplasmic reticulum, the cell surface, and the lysosomal system of the cell. There is probably only one GA per cell, and all stacks of the GA appear to function synchronously. All Golgi apparatus are involved in the generation and movement of product and membrane within the cell or to the cell exterior, and these functions are often reflected as structural changes across the stacks. For example, in plants, both product and membrane appear to maturate from the cis to the trans poles of the stacks in a sequential, or serial, manner. However, there is also strong ultrastructural evidence in plants for a parallel input to the stack saccules, probably through the peripheral tubules. The same modes of functioning probably also occur in animal GA; although here, the parallel mode of functioning almost surely predominates. In some cells at least, GA stacks give rise to tubular-vesicular structures that resemble the trans Golgi network. Rudimentary GA, consisting of tubular-vesicular networks, have been identified in fungi and may represent an early stage of GA evolution.     

Golgi apparatus and golgi zone

The author of this paper has attempted to clarify some problems concerning the nomenclature of Golgi apparatus and Golgi zone. The actual aim of this paper is to summarize — while using the more safe nomenclature—the existing knowledge about the functional relations between nucleus and cytoplasm arising from the study of the juxtanuclear zone by electron microscopy. Some observations lead to the assumption that the juxtanuclear zone is the place where cell components are formed or transformed. Considering its temporary character in proliferating cells and taking into account the connections with endoplasmic reticulum and the presence of pores, the nuclear membrane remains apparently a barrier restraining the spontaneous movement of substances and of cell components respectively between cytoplasm and karyoplasm that can be seen e.g. in the grouping of cytoplasmic formations in the juxtanuclear zone. In plant cells, within the zone mentioned agglomerations of different cell formations have been found, either the Golgi apparatus or mitochondria, secretion granules, lipid inclusions, vacuoles or plastids. Such a gathering of cytoplasmic material has been observed especially in young embryonic cells or in cells with retarded or stopped metabolism. The older and/or intensively active cells would then absolve an expansion of the cytoplasmic material into the whole cell. Similar formative mechanisms, now available for study during some ontogenic phases or at definite functional states only, could be effective even in the course of phylogenesis. From this point of view some of the formations described could be regarded as a kind of atavisms.     

Intercisternal substances of the Golgi apparatus

Summary In media of high ionic strength, neutral pH, low temperature, and varying ion composition, plant dictyosomes were disassembled into component cisternae. The effective ions included phosphotungstate and several halides. Constituents of the intercisternal or bonding regions were revealed through electron microscope analysis. These included intercisternal elements and electrontransparent plaques of undetermined composition. The intercisternal plaques were confined to the central platelike regions of cisternae and were distinct from the intercisternal fibers. The findings demonstrate that plant dictyosomes can be dissociated into component cisternae. With monovalent halide salts, the unstacking process was sufficiently mild to reveal constituents of the intercisternal region as well as yield intact single cisternae.     

The Golgi apparatus: defining the identity of Golgi membranes

The Golgi apparatus is a stack of compartments that serves as a central junction for membrane traffic, with carriers moving through the stack as well as arriving from, and departing toward, many other destinations in the cell. This requires that the different compartments in the Golgi recruit from the cytosol a distinct set of proteins to mediate accurate membrane traffic. This recruitment appears to reflect recognition of small GTPases of the Rab and Arf family, or of lipid species such as PtdIns(4)P and diacylglycerol, which provide a unique "identity" for each compartment. Recent work is starting to reveal the mechanisms by which these labile landmarks are generated in a spatially restricted manner on specific parts of the Golgi.     

Structural organization of the Golgi apparatus

The Golgi apparatus is a universal feature of eukaryotes, carrying out the key functions of processing, sorting and trafficking of newly synthesized membrane and secretory proteins. The Golgi apparatus has a clearly defined structure, comprising stacks of flattened cisternal membranes that in vertebrates are connected to form a ribbon. How this structure is maintained and how it relates to the functions of the Golgi apparatus has long been an area of interest. In this review I describe recent progress in the identification and characterization of the molecular machinery that together help generate the characteristic organization of this organelle.     

The structure and function of the Golgi apparatus: a hundred years of questions

Over the last century, the Golgi apparatus has attracted the attention of researchers world-wide. This highly variable and polymorphic organelle plays a central role in intracellular membrane traffic. Not only does it receive all the secretory material and membrane synthesized by the endoplasmic reticulum and modifies these products by glycosylation, but also packages them and sends them in vesicular carriers to their correct destinations. It is also capable of the synthesis of complex polysaccharides used for building cell walls, a feature unique for higher plants. Yet, the current models of Golgi function are based on those established for yeast and mammalian cells and may not be completely relevant to plants. This review is an attempt to summarize the current knowledge of the plant Golgi apparatus and, where possible, to discuss the applicability of the current models of Golgi function to the plant cell.     

Traffic through the Golgi apparatus.

The role of vesicles in cargo transport through the Golgi apparatus has been controversial. Large forms of cargo such as protein aggregates are thought to progress through the Golgi stack by a process of cisternal maturation, balanced by a return flow of Golgi resident proteins in COPI-coated vesicles. However, whether this is the primary role of vesicles, or whether they also serve to transport small cargo molecules in a forward direction has been debated. Two papers (Martínez-Menárguez et al., 2001; Mironov et al., 2001, this issue) use sophisticated light and electron microscopy to provide evidence that the vesicular stomatitis virus membrane glycoprotein (VSV G)* is largely excluded from vesicles in vivo, and does not move between cisternae, whereas resident Golgi enzymes freely enter vesicles as predicted by the cisternal maturation model. Both papers conclude that vesicles are likely to play only a minor role in the anterograde transport of cargo through the Golgi apparatus in mammalian tissue culture cells.     

Phospholipase D in the Golgi apparatus

Phospholipase D has long been implicated in vesicle formation and vesicular transport through the secretory pathway. The Golgi apparatus has been shown to exhibit a plethora of mechanisms of vesicle formation at different stages to accommodate a wide variety of cargo. Phospholipase D has been found on the Golgi apparatus and is regulated by ADP-ribosylation factors which are themselves regulators of vesicle trafficking. Moreover, the product of phospholipase D activity, phosphatidic acid, as well as its degradation product diacylglycerol, have been implicated in vesicle fission and fusion events. Here we summarize recent advances in the understanding of the role of phospholipase D at the Golgi apparatus.