Ultrastructural observations of the protonephridia of Polymerurus nodicaudus (Gastrotricha: Paucitubulatina)

Kieneke, A. and Hochberg, R. 2012. Ultrastructural observations of the protonephridia of Polymerurus nodicaudus (Gastrotricha: Paucitubulatina). —Acta Zoologica (Stockholm) 93 : 115–124. We studied different regions of the protonephridia of the limnic gastrotrich Polymerurus nodicaudus by means of light and electron microscopy to determine how freshwater species might differ from their marine relatives. Microscopic and ultrastructural characters are in accordance with another limnic species of Paucitubulatina, Chaetonotus maximus, whose protonephridial system has been previously reconstructed. Shared protonephridial characters of both species include the presence of highly elongate terminal organ cilia, microvilli, and the canal cell lumen as well as the presence of a conspicuous anterior loop of the protonephridial lumen. These features are not present in representatives of earlier, marine, paucitubulatan lineages (i.e., Xenotrichulidae) and so are assessed as evolutionary novelties that were likely important for the successful colonization of the freshwater environment.     

Ultrastructure of the lycophora larva of Gyrocotyle urna (Cestoda,Gyrocotylidea)

Summary The ultrastructure of the protonephridial system of the lycophore larva of Gyrocotyle urna Grube and Wagener, 1852, is described. It consists of six terminal cells, at least two proximal canal cells, two distal canal cells and two nephridiopore cells. The terminal cells and the proximal canal cell build up the filtration weir with its two circles of weir rods. The proximal canal cell constitutes a solid, hollow cylinder without a cell gap and desmosome. The distal canal cell is characterized by a strong reduction of the canal lumen by irregularly shaped microvilli. The nephridiopore region is formed by a nephridiopore cell; its cell body is located at some distance proximally within the larva. The connection among different canal cells is brought about by septate desmosomes. Morphological, evolutionary and functional aspects of the protonephridial system within Platyhelminthes are discussed. The structure of the proximal canal cells without a desmosome is considered an autapomorphy of Cestoda.Abbreviations ci cilia of the terminal cell - Co distal canal cell - col lumen of the distal canal cell - Ep epidermis - er outer rods of the filtration weir - il inner leptotriches - ir inner rods of the filtration weir - ld lipid droplets - mt microtubule - mv microvilli - Nc nephridiopore cell - Ne neodermis anlage cells - nu nucleus - pC proximal canal cell - ro ciliary rootlets - sd septate desmosome - Tc terminal cell     

Ultrastructure of the protonephridia of larval Rugiloricus cf. cauliculus, male Armorloricus elegans, and female Nanaloricus mysticus (Loricifera)

The protonephridial system of several Loricifera was studied by transmission electron microscopy. A larval specimen of Rugiloricus cf. cauliculus possesses two protonephridia, which are "capped" frontally by a compact mass of still undifferentiated gonadal cells. Each protonephridium consists of four monociliary terminal cells and four canal cells with a diplosome but no cilia. Because of incomplete series of sections and unsatisfactory fixation, the outleading cell(s) could not be detected. In a male specimen of Armorloricus elegans, each gonad contains two protonephridia that open into the gonadal lumen. Each protonephridium consists of two monociliary terminal cells, each forming a filter, two nonciliated canal cells, and two nephroporus cells. The protonephridial lumina of the latter cells fuse to one common lumen, which unites with the gonadal lumen. Preliminary observations on the protonephridia of a female Nanaloricus mysticus reveal a more complicated arrangement of interdigitating terminal and canal cells. One or two terminal cells form their own individual filter or four cells form a common compound filter. The cilium of the terminal cells of all species investigated are surrounded by a palisade of nine microvilli that support the filter barrier made of an extracellular matrix. An additional filter diaphragm could be traced between the pores in the cell wall of each terminal cell of A. elegans. The urogenital system of the Loricifera differs from that of the Priapulida in that the protonephridia of the former are completely integrated into the gonad, whereas the excretory organs of the latter open into the urogenital duct caudally of the gonads.     

Ultrastructure of the protonephridial system in Neodasys chaetonotoideus (Gastrotricha: Chaetonotida) and in the ground pattern of Gastrotricha

The taxon Neodasys has a basal position within Gastrotricha. This makes it very interesting for phylogenetic considerations in this group. To complete the reconstruction of the nephridial system in the stem species of Gastrotricha started earlier, we have studied the whole protonephridial system of Neodasys chaetonotoideus by means of complete sets of ultrathin sections and TEM. In many characters, protonephridia of N. chaetonotoideus resemble those of macrodasyidan gastrotrich species. For example, each of the six protonephridia, arranged in three pairs, consists of three distinct cells that constitute the continuous protonephridial lumen. Especially, the terminal cell of the protonephridia of N. chaetonotoideus shows a striking pattern: The perforation of the filter region is a meandering cleft that is continuous with the seam of the enfolded lumen of that cell. With the results presented here and that of former TEM studies, we give a comprehensive idea of the excretory organs in the ground pattern of Gastrotricha. Moreover, we can elaborate on the hypothesized protonephridial system in the stem species of Bilateria. We suggest that a meandering filtration cleft is a feature of the ground pattern of the Bilateria.     

Ultrastructure of the Protonephridium in Acteonemertes bathamae Pantin (Rhynchocoela: Enopla: Hoplonemertini)

The protonephridial system consists of terminal cell, protonephridial capillary, protonephridial tubule and efferent duct. The terminal cell is an elongated, thin-walled, fenestrated basket containing a ciliary flame circumscribed by a palisade of straight microvilli. The filtration area is confined to the terminal cell and consists of slits bridged by a filtration membrane. The cilia, as well as the microvilli, projects into the proximal bell-shaped part of the thin-walled protonephridial capillary. The terminal cells are often found in pairs connected to the same capillary, which has a very narrow lumen. The proximal part of the thick-walled, convoluted protonephridial tubule is ciliated and shows characteristic foldings of the luminal plasma membrane and numerous small vesicles in the cytoplasm. The cells of the following, non-ciliated part of the tubule have interdigitating lateral surfaces and the bases deeply invaginated to form compartments with numerous mitochondria; in the cytoplasm are many large vesicles, possibly containing lipid droplets, and small amounts of glycogen. The distal protonephridial tubule resembles various epithelia with an osmoregulatory function, including the vertebrate nephron.     

The Protonephridia of the Arctic Kinorhynch Echinoderes aquilonius (Cyclorhagida,Echinoderidae)

The cyclorhagid kinorhynch Echinoderes aquilonius Higgins & Kristensen, 1988 possesses a single pair of protonephridia located in segments 10 and 11. The protonephridia consist of: (1) three terminal cells T-1, T-2. T-3, each with two cilia; (2) a single non-ciliated canal cell; (3) a nephridiopore cell with many microvilli and a cuticular sieve plate. The protonephridia of Echinoderes are presumed to develop from the ectoderm near the area of the sieve plate on the eleventh segment, and are suspended in the dorso-lateral pseudocoelomic cavity where they are surrounded by a basal lamina. One of the terminal cells (T-1) secondarily penetrates the basal lamina of the tenth segment and a part of the cell attaches to the cuticle. The kinorhynch protonephridia are compared with the excretory organs of other Bilateria. expecially the ‘aschelminths’, and apomorphic characters of the kinorhynch protonephridia are defined.     

Investigations on the protonephridial system of post-larval Gyrocotyle urna and Amphilina foliacea (Cestoda).

The gross morphology and ultrastructure of the different parts of the protonephridial system of the monozoic tapeworms Gyrocotyle urna and Amphilina foliacea are described. The terminal cell in both species has numerous cilia which are interconnected and extend into the lumen of the first canal cell. The filtration area is built up from projections of two cells, the terminal cell and the first canal cell. The first canal cell forms a solid hollow cylinder without a cell gap and a desmosome as found in Neodermata other than cestodes and Udonella. In Gyroctyle the nucleus of the first canal cell is located in the wall cytoplasma whereas more distally located ductules of both species have subepithelial cell bodies containing the nuclei. In both taxa the protonephridial canal system is reticulate. In Amphilina the distal canals lack non-terminal ciliary flames, such ciliary tufts can be found in the larger capillaries of Gyrocotyle. The capillary cilia have rootlets and the ultrastructure of the duct wall cytoplasm containing large numbers of vesicles indicates highly active transport processes. The morphology of the protonephridial systems is discussed with regard to the evolution of Neodermata (especially of the Cestoda) and the function of the protonephridial system in cestodes as a probable organ of nutrient distribution.     

Ultrastructure and significance of the transitory nephridia in Erpobdella octoculata (Hirudinea, Annelida)

In early developmental stages of Erpobdella octoculata two pairs of transitory nephridia occur which degenerate during the formation of the body segments. Because in the ground pattern of Annelida the first nephridia formed during ontogenesis are protonephridia, it can be assumed that the transitory nephridia of E. octoculata are homologous to the larval protonephridia (head kidneys) of Polychaeta. To test this hypothesis two cryptolarvae of E. octoculata were investigated ultrastructurally. Both pairs of transitory nephridia are serially arranged to either side of the midgut vestigium. Each organ consists of a coiled duct that opens separately to the exterior by an intraepidermal nephridiopore cell. The duct is percellular and formed by seventeen cells. Adluminal adherens and septate junctions connect all duct cells; the most proximal duct cell completely encloses the terminal end of the duct lumen. A filtration structure characteristic for protonephridia is lacking. Additionally, the entire organ lacks an inner ciliation. Morphologically and ultrastructurally the transitory nephridia of E. octoculata show far reaching congruencies with the segmental metanephridia in different species of the Hirudinea. These congruencies support the assumption that formation of transitory nephridia and definitive metanephridia in Hirudinea depends on the same genetic information. The same inherited information is assumed to cause the development of larval head kidneys and subsequently formed nephridia in different species of the Polychaeta. Thus, the presumed identical fate of a segmentally repeated nephridial anlage supports the hypothesis of a homology between the transitory nephridia in Hirudinea species and the protonephridial head kidneys in the ground pattern of the Polychaeta. We, therefore, assume that functional constraints lead to a modification of the protonephridial head kidneys in Hirudinea and explain ultrastructural differences between the transitory nephridia in Hirudinea and the protonephridia in Polychaeta. Accepted: 11 December 2000     

The ultrastructure of the protonephridial system of Götte's larva of Stylochus mediterraneus (Polycladida, Platyhelminthes)

The protonephridial system of Götte's larva of Stylochus mediterraneus was studied by electron microscopy. There is one protonephridium on each side of the body, formed by one terminal and one canal cell. The terminal filtration apparatus is formed by a single cell (the terminal cell) with several globular processes, the largest of which includes the nucleus. Fingers of cytoplasm (leptotriches) from each process penetrate the lumen surrounding the bundle of cilia and fingers from adjacent processes interdigitate to form a pattern of convoluted slits which constitute the weir. The single canal cell is inserted internally to the terminal cell at the top of the weir and encloses the lumen without a junction. Septate junctions are present between the terminal and canal cells. The lumen of the canal cell is smooth-walled for most of its length and cilia arise and terminate at all levels of the terminal and canal cells. Posterior to the larval mouth opening, the canal cell crosses the epithelium and the lumen ramifies to form the excretory opening. The terminal apparatus closely resembles that found in the freshwater planarian Bdellocephala brunnea .     

The evolution of the protonephridial terminal organ across Rotifera with particular emphasis on Dicranophorus forcipatus,Encentrum mucronatum and Erignatha clastopis (Rotifera: Dicranophoridae)

Riemann, O. and Ahlrichs, W.H. 2009. The evolution of the protonephridial terminal organ across Rotifera with particular emphasis on Dicranophorus forcipatus, Encentrum mucronatum and Erignatha clastopis (Rotifera: Dicranophoridae). —Acta Zoologica (Stockholm) 91 : 199–211 We report on the ultrastructure of the protonephridial terminal organ in three species of dicranophorid rotifers (Dicranophorus forcipatus, Encentrum mucronatum and Erignatha clastopis). Differences between the three species relate to shape and size, the morphology of the filter region and the number of microvilli and cilia inside the terminal organ. A comparison across Rotifera indicates that the terminal organs in D. forcipatus display a number of plesiomorphic characters, but are modified in E. mucronatum and Er. clastopis. This is in accordance with the results of phylogenetic analyses suggesting a basal position of D. forcipatus compared with the more derived species E. mucronatum and Er. clastopis. Moreover, we survey available data on the terminal organ in Rotifera and discuss its evolutionary transformations. The protonephridial terminal organ in the common ancestor of Rotifera consisted of a cytoplasmic cylinder with cilia united into a vibratile flame and a single circle of circumciliary microvilli. Depending on the topology on which characters are optimized, the site of ultrafiltration was formed by longitudinal cytoplasmic columns spanned by a fine filter diaphragm or by pores in the wall of the terminal organ. In several taxa of Rotifera, the terminal organ – probably independently – lost its circumciliary microvilli.     

Ultrastructure and phylogenetic significance of the head kidneys in <Emphasis Type="Italic">Thalassema</Emphasis><Emphasis Type="Italic">thalassemum</Emphasis> (Thalassematinae,Echiura)

Recent molecular analyses consistently resolve the “spoon worms” (Echiura) as a subgroup of the Annelida, but their closest relatives among annelids still remain unclear. Since the adult morphology of echiurans yields limited insight into their ancestry, we focused on characters of their larval anatomy to contribute to this discussion. Electron microscopical studies of the larval protonephridia (so-called head kidneys) of the echiuran species Thalassema thalassemum revealed distinct correspondences to character states in serpulid polychaetes, although a close relationship between Echiura and Serpulidae is not supported by any phylogenetic analysis. The larval head kidneys of T. thalassemum consist of only two cells, a terminal cell and a duct cell. The terminal cell forms a tuft of six cilia projecting into the lumen of the terminal cell. The cilia are devoid of circumciliary microvilli. A filter structure is formed by two to three layers of elongate microvilli that surround the lumen of the terminal cell in a tubular manner. A thin layer of extracellular matrix (ECM) encloses the outer microvilli of the tubular structure. The tips of the microvilli project into the lumen of the adjacent duct cell but are not directly connected to it. However, mechanic coupling is facilitated by the surrounding ECM and abundant hemidesmosomes. The distal end of the multiciliary duct cell forms the external opening of the nephridium; a specialized nephropore cell is absent. Apart from the multiciliarity of the duct cell, details of the head kidneys in T. thalassemum reveal no support for the current assumption that Echiura is closely related to Capitellida and/or Terebelliformia. Available data for other echiuran species, however, suggest that the head kidneys of T. thalassemum show a derived state within Echiura.     

Ultrastructure of the tubular nephron of the lizard Podarcis (= Lacerta) Taurica

The proximal, intermediate, and distal convoluted tubules of the neprhon of Podarcis (= Lacerta) taurica were examined by electron microscopy. Proximal tubule cells have large, apical cytoplasmic protrusions and microvilli interpreted to function in urate secretion. Adjacent cells are bound apically by tight junctions and desmosomes but interdigitate in their basal region. This situation is repeated in the other tubules with significant differences in intercellular space width. The basal surfaces bear numerous cytoplasmic processes. The intermediate tubule has proximal and distal segments each with dark, ciliated, and light cells, the cuboidal dark cells with dense cytoplasm constituting the main bulk of the wall. As the cells of the proximal and distal segments resemble those of the proximal and distal convoluted tubules, respectively, the intermediate tubule is considered as a transition region. The ciliated cell body has two broad processes extending from the lumen, one to the basement membrane and one to a foot process of a light cell. The light cell is surrounded by dark and ciliated cells. It does not reach the lumen, but contacts the basement membrane through a process running below a ciliated cell to form a mushroom-shaped structure in tubule cross-section, the light cell process forming the stalk and a ciliated cell the cap. The cilia probably propel the glomerular filtrate towards the distal convoluted tubule. This latter tubule has initial, middle, and terminal zones, all nonciliated but with different lumen widths and cell shapes.     

扩张莫尼茨绦虫(绦虫纲:圆叶目)的原肾管及原肾管概念的评述

本研究应用透射电子显微镜研究了扩张莫尼茨绦虫原肾管的细胞学特征 ,莫尼茨绦虫原肾管的焰茎球为一个过滤器结构 ,类似于“挡河坝”样构造 ,此构造由端细胞和近管细胞外突形成的肋条 (或称杆 )相互交错排列而成。肋条之间由细胞外物质构成的“膜”结构连接 ,过滤作用通过该“膜”发生。焰细胞与近管细胞交界处有裂缝或孔与细胞外的结缔组织 (实质组织 )相通 ;原肾管的毛细排泄管细胞质索之间没有隔状联结 ;毛细排泄管及排泄管的管腔内有大量珠状微绒毛突起以增加表面积。从扩张莫尼茨绦虫及其它一些无脊椎动物原肾管的研究结果表明 ,原原肾管概念将焰细胞作为封闭的盲端已不再合适 ,需要进行修订 ,建议修订为 :原肾管是一种焰细胞系统 ,通常由焰细胞、管细胞和肾孔细胞组成 ,焰茎球作为过滤装置与周围的结缔组织 (实质组织 )有或没有裂缝 (孔 )相通     

The fine structure of protonephridia in Gnathostomulida and their comparison within Bilateria

Summary The fine structure of the protonephridia of Haplognathia rosea (Filospermoidea) and Gnathostomula paradoxa (Bursovaginoidea) is described. Each protonephridium consists of three different cells: (1) a monociliated terminal cell which constitutes the filtration area, (2) a nonciliated canal cell showing a special protonephridial outlet system, and (3) an intraepidermal cell — the nephroporus cell — constituting the nephroporus. The protonephridia are arranged serially. There is no canal system connecting the protonephridial units.Protonephridial characters in other Bilateria are considered. The pattern of characters in the protonephridia in the last common gnathostomulid stem species and presumed apomorphies in the protonephridia of the Gnathostomulida investigated are discussed.Abbreviations used in figures ac acessory centriole - AC additional epidermal cell - bb basal body - bl basal lamina - bm bundle of microvilli - c cilium - cc cilium duct cell - cd cilium duct - cr ciliary rootlet - crs structures resembling ciliary rootlets - di diplosome - ds desmosome - dy dictyosome - f filtration area - g granules - m mitochondrium - mv microvillus - n nucleus - NC nephroporus cell - np nephroporus - oc outlet canal - TC terminal cell - tl tubules of lacunar system     

Development of the excretory system in the polyplacophoran mollusc,Lepidochitona corrugata: The protonephridium

A single pair of protonephridia is the typical larval excretory organ of molluscs. Their presence in postlarval developmental stages was discovered only recently. We found that the protonephridia of the polyplacophoran mollusc, Lepidochitona corrugata, achieve their most elaborate differentiation and become largest during the postlarval period. This study describes the protonephridia of L. corrugata using light and electron microscopy and interactive three‐dimensional visualization. We focus on the postlarval developmental period, in which the protonephridia consist of three parts: the terminal part with the ultrafiltration sites at the distal end, the voluminous protonephridial kidney, and the efferent nephroduct leading to the nephropore. The ultrafiltration sites show filtration slits between regularly arranged thin pedicles. The ciliary flame originates from both the terminal cell and the duct cells of the terminal portion. The efferent duct also shows ciliation. The most conspicuous structures, the protonephridial kidneys, are voluminous swellings composed of reabsorptive cells (“nephrocytes”). These cells exhibit strong vacuolization and an infolding system increasing the basal surface. The protonephridial kidneys, previously not reported at such a level of organization in molluscs, strikingly resemble (metanephridial) kidneys of adult molluscan excretory systems. J. Morphol., 2011. © 2011 Wiley‐Liss, Inc.     

Ultrastructure of the protonephridia in Pycnophyes kielensis (Kinorhyncha,Homalorhagida)

Summary Pycnophyes kielensis possesses one pair of protonephridia. The single excretory organ of a female consists of 25 cells: 22 terminal cells, 2 canal cells, and 1 nephroporus cell. Generally, all cells exhibit two cilia, the only exception being the nephroporus cell, which contains a diplosome instead. The slashed peripheral cytoplasmic walls of the 22 terminal cells altogether constitute one compound filter and a common filtration area. The protonephridia discharge via cuticularized cavities and six cuticularized tubes. Two accessory cells with modified cilia penetrate the nephroporus cell. These cells are considered to be receptor cells. The protonephridium of the first juvenile stage of P. kielensis is built up of only 5 cells: 3 terminal cells, 1 canal cell, and 1 nephroporus cell. It opens to the outside via 1 cuticularized tube. The protonephridia within both the Kinorhyncha and the Bilateria are discussed. Presumably excretory organs with compound filters developed independently within Bilateria.Abbreviations bb basal body - c canal cell - ca cuticularized cavity - ci cilium - cu cuticle - d dictyosome - de desmosome - di diplosome - dl dorsal longitudinal muscle - dv dorsoventral muscle - ecm extracellular matrix - ep epidermal cell - ex excretory organ - fc filter cleft - fi filter - fm fastening muscle cell - he hemidesmosome - i intestine - if intercellular fluid - m mitochondrium - mv microvilli - n nephroporus cell - nu nucleus - r ciliary rootlet - re accessory cell (presumable receptor cell) - sj septate junction - t terminal cell - tu cuticularized tube - v vesicle - w peripheral cytoplasmic wall     

Ultrastructure of the nephridio-circulatory connections in Tubulanus annulatus (Nemertini,Anopla)

Summary The protonephridial terminal organs in the nemertean Tubulanus annulatus form an integral part of the blood vessel wall. Both endothelial and muscle-cell layers of the vessel's wall are discontinued at the site of each terminal organ. The terminal organs are usually composed of from one to three terminal cells enclosing a central lumen provided with many microvilli and separated from the blood vessel's lumen by a membranous filtration area. The latter is perforated by numerous winding clefts formed by interdigitation of minute cytoplasmic pedicels arising from processes issued by each of the involved terminal cells. Ultrafiltration of blood plasma takes place across a filtration membrane which spans the cleft system and the basal lamina of the terminal cells. Fluid is propelled into the lumen of the terminal organs through the activity of ciliary bundles, one for each terminal cell involved, perhaps supplemented by vascular turgor. All efferent conduits of the protonephridium have profuse infoldings of the luminal cell surfaces and/or numerous pinocytotic pits suggestive of reabsorption of substances from the primary urine.Abbreviations BL basal lamina - C cilium - CP coated pit - CT collecting tubule - CV inzcoated vesicle - D dictyosome - E endothelial cell - F fenestration of endothelial cell - FA filtration area - FM filtration membrane - G glycogen granule - LV lateral vessel - M mitochondrion - MC muscle cell - MV microvillus - N nucleus of terminal cell - NE nucleus of endothelial cell - NP nephridiopore - PC protonephridial capillary cell - PT protonephridial tubule - R rootlet - TC terminal cell     

Ultrastructure of the protonephridial system of regenerating Stenostomum sp. (Plathelminthes,Catenulida)

Summary The ultrastructure of the flame bulbs, protonephridial capillaries and duct of fully developed and regenerating Stenostomum sp. is described. Flame bulbs are formed by a single cell whose nucleus is located basally or laterally to the weir. The weir is formed by a single row of transverse ribs connected by a thin membrane, apparently of extracellular matrix. Internal leptotriches arise from the proximal cytoplasm and extend in a (usually) single row along the weir and into the lumen of the distal cytoplasmic tube. Many or all leptotriches do not fuse with the distal cytoplasm. Two cilia are each anchored in the proximal cytoplasm by a cross-striated vertical and lateral rootlet, the latter bent forward and extending for some distance into one of the two cytoplasmic cords along the weir. Each cord contains the lateral rootlet in its proximal part, as well as many microtubules. The distal cytoplasmic tube contains two (longitudinal) junctions, i.e. lines of contact between cell processes of the same, terminal cell. Occasionally, more than two junctions were seen, apparently due to branches of the terminal cell in contact with each other. Flame bulbs join capillaries lined by several canal cells type I, containing few or no microvilli but lateral flames. Such capillaries join a duct (or ducts?) lined by canal cells type II with many long microvilli. The large protonephridial duct is lined by numerous cells with lateral flames and many long microvilli. In regenerating tissue (10.5 hours after cutting) some flame bulbs were free, i.e. not connected to capillaries, and some capillaries openly communicated with the surrounding intercellular space. In the presence of a single row of ribs in the weir, of internal leptotriches, and of vertical and lateral ciliary rootlets, the flame bulb of Stenostomum sp. resembles that of other Plathelminthes much more closely than hitherto thought. The species differs from non-catenulid plathelminths mainly in the large number of glandular cells lining the large protonephridial ducts, in the transverse orientation of the ribs in the weir and in the presence of only two cilia in the flame.     

No direct contact between the excretory system and the circulatory system in Prostomatella arenicola Friedrich (Hoplonemertini)

Excretory and circulatory systems in Prostomatella arenicola are examined at the ultrastructural level. Interdigitating cells, which rest on a thin fibrillar basal lamina, line the lumina of the lateral vessels. A layer of muscle cells and an underlying sheath of fibrillar extracellular material surround each vessel.The excretory system consists of one pair of laterally situated branched protonephridia. Each protonephridium is composed of several terminal cells, an efferent duct and a nephridiopore. The terminal parts of the protonephridia are not restricted to the vicinity of the circulatory system; they can also be found dorsally or laterally to the nerve cords between muscle cells. The presumed filtration area arises as a hollow cylinder from the terminal cell. This cylinder is perforated by numerous clefts which are never bridged by a filter diaphragm. Instead, each terminal cell cylinder is surrounded by an extracellular matrix. The terminal cells neither extend into the lumen of the lateral vessel nor contact the vessel lining cells.Phylogenetic implications of the results are discussed.     

The fine structure of the protonephridial system in the land nemertean Pantinonemertes californiensis (Rhynchocoela,Enopla, Hoplonemertini)

Summary The protonephridial terminal organ in the nemertean Pantinonemertes californiensis is composed of two cells that are similar in size and shape and are mirror images of each other. Basally in the organ the two cells combine to form a binucleate cytoplasmic mass. Apically they are intimately joined to form a subcylindrical thin-walled weir apparatus; this part is supported by two opposed cytoplasmic columns running the length of the weir region, one originating from each of the two cells, and by a number of regularly spaced circular bars that arise from the two columns. The ciliary flame consists of 94–114 cilia that originate in the bases of the two cells, and it is surrounded by a palisade of incomplete circlets of long, straight microvilli. The convoluted protonephridial tubule is rich in structures that indicate intensive reabsorption from the primary urine. It is argued that the terminal organs in Pantinonemertes and Geonemertes are fundamentally similar and differ only in the amount of microtubules present in the longitudinal supports.Abbreviations BL basal lamina - CF ciliary flame - CT connective tissue - CV coated vesicle - E endocytotic pit - FM filtration membrane - G Golgi complex - LC longitudinal cytoplasmic column - M mitochondrion - MT microtubules - MV microvilli - N nucleus - NPC nucleus of protonephridial capillary cell - PC protonephridial capillary cell - R rootlets - TB transverse bar - TC terminal cell - WE weir, exterior of fenestrated wall - WI weir, interior of same