Changes in microtubule packing during the stretching of an extensible microtubule bundle in the ciliate Nassula

Summary The cytopharyngeal sheath in the ciliate Nassula is a long hollow tube-shaped microtubule bundle that forms part of a large feeding organelle called the cytopharyngeal basket. During the initial stages of ingestion of algal filaments by Nassula the sheath is stretched, becomes approximately elliptical in cross-section, and its external cross-sectional perimeter increases by a factor of about two. The mean circumferential centre-to-centre spacing of radially oriented rows of sheath tubules increases from 57 to 137nm during stretching but sheath thickness and the radial spacing of sheath tubules do not change appreciably. It is suggested that extensible circumferentially oriented intertubule links and relatively inextensible radial links may define the anisometric mechanical properties of this particular microtubule bundle which are related to its cytoskeletal role. The possibility that extensible links resist stretching elastically and provide the restoring forces for return of the sheath to its former shape and dimensions after stretching is considered.Supported by the Science Research Council, U.K. (Grant nos. B/RG/5894.5 and GR/A/0875.8)     

The ultrastructure of the mid-gut cells of Nasonia vitripennis (Walker) (Hymenoptera,Pteromalidae)

Summary The ultrastructure of the mid-gut cells of female Nasonia vitripennis is described. The mid-gut consists of a uniform, single-cell epithelium. The cells of different gut regions were analysed using morphometric techniques in order to determine any differences in the components. The structure of the cells is described in the unfed animal, and after varying periods of feeding on host body-fluids. Tissues were sampled after 12 h and 24 h of feeding on host body-fluids and after 24 h feeding/24 h starvation. The cells were found to be complex and contain an organelle component that allows solute-transport and extensive lipid synthesis. A limited cytochemical analysis involving the lysosomal marker enzyme-acid phosphatase — and the respiratory enzyme — cytochrome oxidase was carried out.We are indebted to Professor E.W. Knight-Jones, in whose Department this work was carried out, and to the Science Research Council for financial support to one of us (I.D.)     

The Formation and Fate of Tetrahymena patula Cryptostomes

A reliable method for producing reproductive cysts in Tetrahymena patula is described. The procedure involves the isolation of macrostomes without cytopharyngeal pouches in microdrops of distilled water under oil. The study of silver-impregnated specimens has shown that a complex pattern of oral resorption and reformation occurs within the cyst that leads to the formation of a group of small cells with recessed oral apparatuses. These cells, called “cryptostomes,” swim very rapidly on excystment and are incapable of either feeding or reproducing. They are presumably dispersal forms. Oral morphogenesis during the transformation of excysted cryptostomes into microstomes and macrostomes is also described.     

The core of the mammalian centriole contains γ-tubulin

Background: The microtubule network, upon which transport occurs in higher cells, is formed by the polymerization of α and β tubulin. The third major tubulin isoform, γ tubulin, is believed to serve a role in organizing this network by nucleating microtubule growth on microtubule-organizing centers, such as the centrosome. Research in vitro has shown that γ tubulin must be restored to stripped centrioles to regenerate the centrosomal functions of duplication and microtubule nucleation.Results We have re-examined the localization of γ tubulin in isolated and in situ mammalian centrosomes using a novel immunocytochemical technique that preserves antigenicity and morphology while allowing increased accessibility. As expected, α tubulin was localized in cytoplasmic and centriolar barrel microtubules and in the associated pericentriolar material. Foci of γ tubulin were observed at the periphery of the organized pericentriolar material, as reported previously, often near the termini of microtubules. A further and major location of γ tubulin was a structure within the proximal end of the centriolar barrel. The distributions were complementary, in that α tubulin was excluded from the core of the centriole, and γ tubulin was excluded from the microtubule barrel.Conclusion We have shown that γ tubulin is localized both in the pericentriolar material and in the core of the mammalian centriole. This result suggests that γ tubulin has a role in the centriolar duplication process, perhaps as a template for growth of the centriolar microtubules, in addition to its established role in the nucleation of astral microtubules.     

Immunocytochemical study of tubulin in the 9+‘1’ sperm axoneme of a monogenean (Platyhelminthes), Pseudodactylogyrus sp.

The spermatozoon of the monopisthocotylean monogenean Pseudodactylogyrus sp. (a gill parasite of eels) has a single axoneme showing a 9+‘1’ pattern, a nucleus and a mitochondrion, but has no cortical microtubules. This species thus provides a very simple model for the study of tubulin in the 9+‘1’ axonemes of the Platyhelminthes, in contrast with digenean sperm which have a more complex spermatozoon with two such axonemes and cortical microtubules. Indirect immunofluorescence labelling of tubulin shows that the elongating spermatids, initially lying in all directions in the early stages, are arranged as parallel elements in further stages. The number of spermatids in an isogenic group could also be precisely counted and equals 32. Nuclear labelling with fluorescent dyes shows that the nuclei, first located in the common mass of the spermatids, later elongate and migrate into the growing spermatids, and that the nucleus is located in the central part of the mature spermatozoon, with the two extremities devoid of nucleus. Labelling with antibodies directed against acetylated, tyrosinated, and polyglutamylated tubulin gave positive results, thus indicating that these post-translational modifications of tubulin are present in the axoneme of spermatids and spermatozoa of monopisthocotylean monogeneans.     

Further investigations of the primary mechanism of benzimidazole resistance in Haemonchus contortus

The binding of the [³H] benzimidazole carbamates (BZCs)—albendazole (ABZ), oxibendazole (OBZ), parbendazole (PBZ), mebendazole (MBZ), fenbendazole (FBZ) and oxfendazole (OFZ)—to tubulin from three ecologically-related isolates of adult Haemonchus contortus has been examined. The extent of binding of each BZC was inversely proportional to the known resistance status of the isolate. Biochemically, the change in the formation of the BZC-tubulin complex was due to a reduction in the amount of drug bound to resistant tubulin, with no significant change in the association constant of the complex. The resistance factors derived from the binding data support the hypothesis that the complex is ligand-dependent, with the aryl-substituted BZCs—MBZ, OFZ and FBZ—demonstrating lower resistance factors than those of the alkyl-substituted BZCs—ABZ, OBZ and PBZ. Examination of the slope derived from plots of binding against protein concentration demonstrated that the failure of resistant or partially resistant isolates to bind was due to either a decrease in the number of binding sites or, more likely, to reduced stability of the BZC-tubulin complex rendering it unstable to charcoal extraction.     

Electron Microscopic Localization of ATPase Activity in the Cytopharyngeal Basket of the Ciliate Pseudomicrothorax dubius

The cytopharyngeal basket of Pseudomicrothorax dubius is used to ingest filamentous blue-green algae. The basket has three main components: a sheath of microfilaments, bundles of microtubules (the nemadesmata), and ribbons of microtubules. The ribbons of microtubules (nemadesmal lamellae) are adpressed to the food vacuole during ingestion. Cytochemical techniques show that both the lamellae and the microfilamentous sheath possess ATPase activity, but the reaction product appears under different conditions in the two cases. The presence of ATPase activity within the microtubular lattices of the feeding organelle suggests the capacity for active motility. Consequently the basket seems to have two motile systems, one may be used to constrict and dilate the cytopharynx while the other is used in the inward propulsion of the forming food vacuole.     

Changes in Oral Apparatus Structure Accompanying Vacuolar Formation in the Macrostomal Form of Tetrahymena vorax. A Model for the Formation of Food Vacuoles in Tetrahymena1

The large cytopharyngeal pouch of the macrostomal form of Tetrahymena vorax, following the addition of calcium, can form a sealed, empty vacuole. The open cytostomal region of this cell, which averages about 16 μ in diameter, is closed by an upward (ventral) movement of the right and posterior ribbed walls, both of which project into the cytostomal cavity. At the same time, the anterior and left walls of the cytostome-cytopharyngeal complex move to the right, forming a diagonally (right to left) placed furrow in the floor of the buccal cavity as these walls meet. As a result of the movement, the edges of the single membrane-bounded cytopharyngeal pouch are brought together and fuse, producing the closed vacuole. Elements of the cytoskeleton appear to participate in the closure process. Three major groups of ribbed wall microtubules support the open cytostome. The anterior ribbed wall microtubules pass laterally along the anterior (dorsal) portion of the cytopharyngeal pouch to the left where they end in the specialized cytoplasm. Middle oral rib microtubules terminate at the right and posterior margin of the cytopharynx while microtubules from the most posterior region of the ribbed wall pass to the left terminating in the specialized cytoplasm. The fine filamentous reticulum, a striated reticulum that borders the right, posterior, and anterior margins of the cytostome-cytopharyngeal complex, is in an ideal position to participate in these movements. It is anchored anteriorly high up in the buccal cavity to the cross-connective between the third membranelle and the undulating membrane complex. It courses beneath the right and posterior ribbed walls and runs laterally along the anterior margin of the cytopharynx to the left side. Contraction or pulling of this reticulum would act to bring the microtubule-reinforced walls of the cytopharynx together permitting fusion of the cytopharyngeal pouch membranes to form a sealed vacuole.     

Identification of tubulin isoforms in different tissues of Ascaris suum using anti-tubulin monoclonal antibodies

Three monoclonal antibodies specific to α- and β-tubulin were used to examine the expression of tubulin isofoms in the intestine, reproductive tract and body wall muscle of A. suum. The tubulins were found to be different in their isoelectric points, number of isoforms and peptide maps with Western blot analysis of one-dimensional polyacrylamide gel confirming the presence of α-, β₁- and β₂- tubulin. Commercial cross-reactive anti-α and anti-β MAbs 356 and 357 recognized tubulin from A. suum tissues as well as from pig brain, whereas anti-A. suum β-tubulin specific MAb P3D6 recognized tubulin from the A. suum tissues only. Two-dimensional gel analysis showed different isoform patterns in different A. suum tissues with anti-A. suum β-tubulin MAb P3D6 and cross-reactive β-tubulin MAb 357 recognizing 2–4 β- tubulin isoforms and anti-α-tubulin MAb 356 recognizing 1–6 α-tubulin isoforms. Different peptide maps of tubulin were observed in the three tissues, when subjected to limited proteolysis followed by SDS-PAGE. The data indicate that different tubulins are found in different tissues of adult A. suum.     

Distribution and Characteristics of βII Tubulin-Enriched Microtubules in Interphase Cells

We have used a polyclonal antibody (Ab196) that specifically recognizes the βII tubulin isotype to examine the subcellular distribution and properties of microtubules enriched in this isotype. Antibody specificity was tested by a method that involves the analysis of its interaction with individual β isotypes. Using photoimaging analysis, we observed βII tubulin-enriched microtubules in the perinuclear region, as well as in the microtubules close to the periphery of interphase cells. The observed sorting of βII-enriched microtubules together with the reported increased levels of βII tubulin in taxol-resistant cells (M. Haberet al.,1995,J. Biol. Chem.270, 31269–31275) prompted us to study the behavior of microtubules enriched in this isotype after different depolymerizing treatments. After cold or nocodazol treatments, βII-enriched microtubules anchored at the centrosome and at the cell periphery were observed. In addition, cold-resistant microtubules were marked mainly by the specific anti-βII tubulin antibody but not by anti-acetylated α tubulin, suggesting the presence of different stable microtubule subsets enriched in particular tubulin isoforms.     

Resistance of Rosa microtubule polymerization to colchicine results from a low-affinity interaction of colchicine and tubulin

The inhibition of the polymerization of tubulin from cultured cells of rose (Rosa. sp. cv. Paul's scarlet) by colchicine and the binding of colchicine to tubulin were examined in vitro and compared with data obtained in parallel experiments with bovine brain tubulin. Turbidimetric measurements of taxol-induced polymerization of rose microtubules were found to be sensitive and semiquantitative at low tubulin concentrations, and to conform to some of the characteristics of a nucleation and condensation-polymerization mechanism for assembly of filamentous helical polymers. Colchicine inhibited the rapid phase of polymerization at 24°C with an apparent inhibition constant (K _i) of 1.4·10^-4 M for rose tubulin and an apparent K _i=8.8·10^-7 M for brain tubulin. The binding of [³H]colchicine to rose tubulin to form tubulin-colchicine complex was mildly temperature-dependent and slow, taking 2–3 h to reach equilibrium at 24°C, and was not affected by vinblastine sulfate. The binding of [³H]colchicine to rose tubulin was saturable and Scatchard analysis indicated a single class of low-affinity binding sites having an apparent affinity constant (K) of 9.7·10² M^-1 and an estimated molar binding stoichiometry (r) of 0.47 at 24°C. The values for brain tubulin were K=2.46·10⁶ M^-1 and r=0.45 at 37°C. The binding of [³H]colchicine to rose tubulin was inhibited by excess unlabeled colchicine, but not by podophyllotoxin or tropolone. The data demonstrate divergence of the colchicine-binding sites on plant and animal tubulins and indicate that the relative resistance of plant microtubule polymerization to colchicine results from a low-affinity interaction of colchicine and tubulin.Abbreviations MT microtubule - TC tubulin-colchicine complex     

Structural basis of tubulin tyrosination by tubulin tyrosine ligase

Tubulin tyrosine ligase (TTL) catalyzes the post-translational retyrosination of detyrosinated α-tubulin. Despite the indispensable role of TTL in cell and organism development, its molecular mechanism of action is poorly understood. By solving crystal structures of TTL in complex with tubulin, we here demonstrate that TTL binds to the α and β subunits of tubulin and recognizes the curved conformation of the dimer. Biochemical and cellular assays revealed that specific tubulin dimer recognition controls the activity of the enzyme, and as a consequence, neuronal development. The TTL–tubulin structure further illustrates how the enzyme binds the functionally crucial C-terminal tail sequence of α-tubulin and how this interaction catalyzes the tyrosination reaction. It also reveals how TTL discriminates between α- and β-tubulin, and between different post-translationally modified forms of α-tubulin. Together, our data suggest that TTL has specifically evolved to recognize and modify tubulin, thus highlighting a fundamental role of the evolutionary conserved tubulin tyrosination cycle in regulating the microtubule cytoskeleton.     

Centriole Disassembly In Vivo and Its Effect on Centrosome Structure and Function in Vertebrate Cells

Glutamylation is the major posttranslational modification of neuronal and axonemal tubulin and is restricted predominantly to centrioles in nonneuronal cells (Bobinnec, Y., M. Moudjou, J.P. Fouquet, E. Desbruyères, B. Eddé, and M. Bornens. 1998. Cell Motil. Cytoskel. 39:223–232). To investigate a possible relationship between the exceptional stability of centriole microtubules and the compartmentalization of glutamylated isoforms, we loaded HeLa cells with the monoclonal antibody GT335, which specifically reacts with polyglutamylated tubulin. The total disappearance of the centriole pair was observed after 12 h, as judged both by immunofluorescence labeling with specific antibodies and electron microscopic observation of cells after complete thick serial sectioning. Strikingly, we also observed a scattering of the pericentriolar material (PCM) within the cytoplasm and a parallel disappearance of the centrosome as a defined organelle. However, centriole disappearance was transient, as centrioles and discrete centrosomes ultimately reappeared in the cell population.During the acentriolar period, a large proportion of monopolar half-spindles or of bipolar spindles with abnormal distribution of PCM and NuMA were observed. However, as judged by a quasinormal increase in cell number, these cells likely were not blocked in mitosis.Our results suggest that a posttranslational modification of tubulin is critical for long-term stability of centriolar microtubules. They further demonstrate that in animal cells, centrioles are instrumental in organizing centrosomal components into a structurally stable organelle.     

Tubulin synthesis in a temperature-sensitive mutant of Chlamydomonas reinhardii

A temperature-sensitive mutant (TSF-1) of Chlamydomonas reinhardii which exhibits altered regulation of tubulin synthesis has been isolated. This mutant grows equally well at permissive (25 °C) and non-permissive (36 °C) temperatures but possesses flagella only at 25 °C. As with wild-type cells, when flagella are detached by ‘pH shock’ at 25 °C there is a rapid regeneration of flagella and a marked induction of tubulin synthesis, the major flagellar protein. However, if flagella are removed at 25 °C and the cells immediately placed at 36 °C, there is little or no flagellar regeneration or tubulin induction. If these flagella-less cells are maintained at 36 °C and subsequently shifted back to 25 °C, there is a rapid initiation of both flagellar outgrowth and tubulin synthesis.An additional temperature-sensitive phenotype exhibited by TSF-1 when shifted from 25 to 36 °C is a spontaneous detachment of flagella. Associated with the loss of flagella is limited (but perhaps repeated) flagellar regeneration and a marked increase in tubulin synthesis. Interestingly, ‘pH shock’ treatment at 30 or 60 min after the shift to 36 °C results in a rapid de-induction of tubulin synthesis. This complements the observation that flagellar excision by ‘pH shock’ just prior to a shift to 36 °C results in little or no tubulin induction. Taken together these results suggest that two independent pathways for tubulin induction may be operable in TSF-1.The short response times observed in both the shift-up and shift-down experiments demonstrate that the conditional process involved responds very rapidly to both positive and negative temperature changes and, moreover, indicate that this process may be intimately associated with the regulation of both flagellar regeneration and flagellar tubulin synthesis.     

Dynamic Subunit Exchange and the Regulation of Microtubule Assembly by the Stress Response Protein Human αB Crystallin

Background

The small heat shock protein (sHSP), human αB crystallin, forms large, polydisperse complexes that modulate the tubulin-microtubule equilibrium using a dynamic mechanism that is poorly understood. The interactive sequences in αB crystallin for tubulin are surface exposed, and correspond to interactive sites for the formation of αB crystallin complexes.

Methodology/Principal Findings

There is sequence homology between tubulin and the interactive domains in the β8-strand of the core domain and the C-terminal extension of αB crystallin. This study investigated the hypothesis that the formation of tubulin and αB crystallin quaternary structures was regulated through common interactive domains that alter the dynamics of their assembly. Size exclusion chromatography (SEC), SDS-PAGE, microtubule assembly assays, aggregation assays, multiple sequence alignment, and molecular modeling characterized the dynamic response of tubulin assembly to increasing concentrations of αB crystallin. Low molar ratios of αB crystallin∶tubulin were favorable for microtubule assembly and high molar ratios of αB crystallin∶tubulin were unfavorable for microtubule assembly. Interactions between αB crystallin and unassembled tubulin were observed using SEC and SDS-PAGE.

Conclusions/Significance

Subunits of αB crystallin that exchange dynamically with the αB crystallin complex can interact with tubulin subunits to regulate the equilibrium between tubulin and microtubules.     

Quantitative study of organelle nucleoids during the second pollen grain mitosis inOenothera biennis

Summary The behavior of organelle nucleoids in the generative cell was examined at the second (pollen grain) mitosis by epifluorescence microscopy after staining with 4,6-diamidino-2-phenylindole (DAPI) inOenothera biennis. TheO. biennis generative cell contained a large number of organelle nucleoids distributed randomly in the cytoplasm before mitosis. The epifluorescence images of the nucleoids could be classified distinctly into two groups which corresponded to plastid nucleoids (pt-nucleoids) and mitochondrial nucleoids (mt-nucleoids). Discrimination between pt- and mt-nucleoids was carried out with the aid of DNA immunogold electron microscopy. At metaphase, both pt- and mt-nucleoids migrated to the pole regions of the generative cell. After mitosis, organelle nucleoids in both of the sperm cells scattered in the cytoplasm again. A quantitative examination of pt-nucleoids on 202 pairs of sperm cells showed that the leading sperm cell (Svn) contained 0–39 pt-nucleoids (19.0 ± 7.4) and the trailing sperm cell (Sua) contained 0–40 pt-nucleoids (15.4 ± 6.5). For mt-nucleoids, examination of 28 pairs of sperm cells showed that Svn contained 5–32 mt-nucleoids (14.5 ± 6.8) and Sua contained 6–30 mt-nucleoids (13.4 ±7.5). These results showed that (1) the number of organelle nucleoids per sperm cell varied considerably in the cells studied; (2) quantitative difference in pt- and mt-nucleoids between Svn and Sua could occur in some gametophytes studied; but (3) it was unlikely that there was any pre-differentiational cytoplasm localization and essential sperm heteromorphy with respect to organelle nucleoid content in the gametophyte population.     

The cytoskeleton of the giant coenocytic green algaCaulerpa visualized by immunocytochemistry

Summary A microdissection technique is described allowing immunocytochemical procedures in the giant coenocytic green algaCaulerpa without the necessity to enzymatically digest the cell wall. In this way, a plant cell famous for its fast, large scale organelle transport becomes available for cytoskeletal research. Using antibodies against tubulin and actin three cytoplasmic levels can be identified in the cell area of the assimilatory blade, each with a distinct cytoskeletal organization. Microtubules run axially through the cortex, form bundles with increasing complexity in the subcortex and combine to giant composite bundles in the center. Actin is detected for the first time inCaulerpa in the form of fine cortical fibers and filamentous foci. The potentials of the new technique for studies on cytskeletal functions in organelle transport, polarity, and cell differentiation inCaulerpa are emphasized.     

How is the flagellar length of mature sperm determined? : II. Comparison of tubulin synthesis in spermatids between newt and Xenopus in vitro

In order to elucidate mechanisms that control flagellar length of mature sperm, we studied in synchronous cell suspension cultures flagellar growth, tubulin pool, and tubulin synthesis in round spermatids of Xenopus laevis and the newt Cynops pyrrhogaster. The average final length of flagella in Xenopus round spermatids was 35 μm, almost the same length as that in mature sperm, whereas in the newt round spermatids, the length was 210 μm, almost half that of mature sperm. Kinetics of flagellar growth showed that the rate and period of flagellar growth in the newt spermatids were two to threefold those in Xenopus spermatids. The tubulin pool size in newt spermatids was estimated to be about 10-fold greater than that in Xenopus spermatids. But even if all of the pool was used for flagellar growth, it could support only about a seventh to a tenth of the flagellar length in mature sperm in either species. Thus, the possibility that the tubulin pool primarily determines flagellar length was excluded. Since the tubulin pool size did not change throughout the culture period, the possibility that the termination of flagellar growth is due to the exhaustion of the tubulin pool was also excluded. Tubulin synthesis declined over the culture period but continued in newt spermatids longer than in Xenopus spermatids. The period of flagellar elongation almost coincided with the period of tubulin synthesis. The amount of rRNA did not decrease, excluding the possibility that the decline of tubulin synthesis was due to cytoplasmic shedding which might result in the loss of ribosomes. Tubulin synthesis and the amount of rRNA in newt spermatids was more than threefold greater than that in Xenopus spermatids, which may explain the difference in growth rates of their flagella.     

Xgrip109: A γ Tubulin–Associated Protein with an Essential Role in γ Tubulin Ring Complex (γTuRC) Assembly and Centrosome Function

Previous studies indicate that γ tubulin ring complex (γTuRC) can nucleate microtubule assembly and may be important in centrosome formation. γTuRC contains approximately eight subunits, which we refer to as Xenopus gamma ring proteins (Xgrips), in addition to γ tubulin. We found that one γTuRC subunit, Xgrip109, is a highly conserved protein, with homologues present in yeast, rice, flies, zebrafish, mice, and humans. The yeast Xgrip109 homologue, Spc98, is a spindle–pole body component that interacts with γ tubulin. In vertebrates, Xgrip109 identifies two families of related proteins. Xgrip109 and Spc98 have more homology to one family than the other. We show that Xgrip109 is a centrosomal protein that directly interacts with γ tubulin. We have developed a complementation assay for centrosome formation using demembranated Xenopus sperm and Xenopus egg extract. Using this assay, we show that Xgrip109 is necessary for the reassembly of salt-disrupted γTuRC and for the recruitment of γ tubulin to the centrosome. Xgrip109, therefore, is essential for the formation of a functional centrosome.     

Five new species of Trichostomatida (ciliated protozoa) from the colon of wild African rhinoceroses

Five new species of Charonina Strand, 1928 were revealed, in addition to 41 species of 20 other apparent genera, in a survey of ciliated intestinal protozoan endocommensals of both black and white wild African rhinoceroses. Charonina species infected the ventral and dorsal region of the ascending colon, where the average total protozoan populations (× 10³/ml digesta fluid) were 100 and 80, respectively, in the white and 270 and 260, respectively, in the black rhinoceroses. Charonina species constituted up to 50% in the ventral and 25% in the dorsal populations. Measurements in micrometres and specific characteristics of the five species are: C. odontophora n. sp. length 70±5.7, width 32±7.2, dorso-ventral thickness 7±1.1, slender ovate-lanceolate-shaped body with frontal lobe and prong-like protrusion in oral-opening; C. tortuosa n. sp. length 87±9.3, width 42±5.3, dorso-ventral thickness 15±2.7, body-shape ovate-lanceolate without frontal lobe, oral-opening with longitudinal ridge, cytopharyngeal canal with sharp bend after emerging from oral-opening; C. dicerotis n. sp. length 67±8.6, width 37±4.0, dorso-ventral thickness 12±2.2, body-shape ovate-lanceolate without frontal lobe, oral-opening without ridge, cytopharyngeal canal curved without sharp bend; C. tenuis n. sp. length 56±10.0, width 16±4.1 at anterior end and 10±2.7 at posterior end, dorso-ventral thickness 7±1.2 at anterior end and 5±1.1 at posterior end, body-shape cone-like with longitudinal striations and frontal lobe; C. tetragona n. sp. length 58±4.7, width 26±3.2, dorso-ventral thickness 12±1.8, body-shape rectangular with frontal lobe and caudal flaps. The length, width and dorso-ventral thickness of the five species are on average in the approximate ratio of 6:3:1, thus showing them to be dorso-ventrally compressed. The body conformation of C. tetragona n. sp. closely resembles that of Didesmis quadrata Fiorentini, 1980, but is distinguished from the latter by the absence of a concrement vacuole and the presence of an elongate cytopharyngeal canal.