Adrenocorticotropin-Like Immunoreactivity in the Granules of Neural Complex Cells of the Ascidian Halocynthia roretzi

Genri Kawahara; Kiyoshi Terakado; Toshio Sekiguchi; Kinji Inoue; Sakae Kikuyama

doi:10.2108/zsj.19.1061

How to translate text using browser tools

1 September 2002 Adrenocorticotropin-Like Immunoreactivity in the Granules of Neural Complex Cells of the Ascidian Halocynthia roretzi

Genri Kawahara, Kiyoshi Terakado, Toshio Sekiguchi, Kinji Inoue, Sakae Kikuyama

Author Affiliations +

Zoological Science, 19(9):1061-1065 (2002). https://doi.org/10.2108/zsj.19.1061

Abstract

Immunohistochemical studies on the neural complex (neural gland, dorsal strand, and cerebral ganglion) of an ascidian, Halocynthia roretzi, were performed by using an antiserum against porcine ACTH. The antiserum recognized a considerable number of the cells scattered along the tubular structure of the dorsal strand and a few cells in the cerebral ganglion. Immunoelectron microscopic studies revealed that the ACTH-like substance resided within secretory granules with diameter of 300–500 nm. Furthermore, those ACTH-immunoreactive cells were demonstrated to be different from PRL-immunoreactive cells, the presence of which had previously been reported.

INTRODUCTION

Several series of experimental studies have demonstrated that the hypophysis in vertebrates from amphibians to mammals is of neuroectodermal origin (Couly and Le Douarin 1985, 1987; Eagleson et al., 1986; Kawamura and Kikuyama 1992; Kouki et al., 2001). This suggests that cells equivalent to the vertebrate adenohypophyseal cells in protochordates, if any, might be found in neuroectodermal derivatives. In ascidians, the neural complex (neural gland, cerebral ganglion, and dorsal strand) is known to be derived from the embryonic neural tube during metamorphosis (Dodd and Dodd 1966).

There are a few earlier reports describing the presence of substances immunoreactive with antisera against pituitary hormones such as prolactin (PRL; Fritsch et al., 1982; Pestarino 1983) and adrenocorticotropic hormone (ACTH; Georges and Dubois 1979, 1985; Pestarino 1988) in the cerebral ganglion of ascidians. However, it has not been examined whether these immunoreactive substances exist within secretory granules. Recently we demonstrated the presence of PRL-immunoreactive substance within the secretory granules in the cells of the dorsal strand as well as in the neuronal cells in the cerebral ganglion of Halocynthia roretzi (Terakado et al., 1997).

As one step to search for the prototype of the vertebrate pituitary, the present experiment was conducted to see whether ACTH- immunoreactive substance exists, as in the case of PRL-like substance, in the cells of the cerebral ganglion and/or the dorsal strand of Halocynthia roretzi, and if so, whether the substance is contained in cells different from the PRL-immunoreactive cells and whether it is localized in the secretory granules.

MATERIALS AND METHODS

Animals

Adult specimens of the ascidian Halocynthia roretzi (weighing 250–450 g) that had been cultured in Mutsu Bay in Aomori City, Japan were purchased from a commercial dealer.

Immunohistochemistry

The neural complexes were excised, fixed with Bouin's fluid without acetic acid for 15 hr, dehydrated through an ethanol series, and embedded in Paraplast. Sections (6 μm in thickness) were mounted on gelatin-coated slides and stained immunohistochemically by the ABC (streptavidin-biotin-peroxidase) method using a polyclonal rabbit antibody against porcine ACTH (Tanaka and Kurosumi, 1986) or bullfrog PRL (Yamamoto and Kikuyama, 1982). Dewaxed and rehydrated sections were treated with 0.5% H₂O₂ in 70% ethanol for 30 min to block endogenous peroxidase activity, washed, and treated with normal swine serum (1: 50; Dako, Copenhagen, Denmark) for 30 min to reduce non-specific staining. The primary antisera against ACTH and PRL, diluted 1: 2000 and 1: 1000, respectively, in 0.01 M phosphate-buffered saline (PBS) containing 0.1% bovine serum albumin (BSA), pH 7.5, were reacted with the sections overnight at 4°C. Biotinylated swine antibody against rabbit immunoglobulins (1: 300; Dako) and peroxidase-conjugated streptavidin (1: 300; Dako) were applied successively, each for 1 hr at room temperature. Immunoreactivity was visualized by exposing the sections to 0.02% 3,3′-diaminobenzidine containing 0.006% H₂O₂ in 0.05 M Tris-HCl buffer (pH 7.5) at room temperature for 3-10 min, after which the sections were stained lightly with Mayer's hematoxylin. Control staining was carried out by incubating sections overnight at 4°C in antiserum against ACTH (1: 2000, 1 ml) or antiserum against PRL (1: 1000, 1 ml) that had been preabsorbed with the corresponding antigen (10 μg).

Immunoelectron microscopy

Dissected neural complexes were cut into small pieces and fixed with 4% paraformaldehyde and 0.5% glutaraldehyde in 0.2 M phosphate buffer (pH 7.2) for 4 hr at 4°C. These tissue pieces were washed overnight at 4°C in 0.1 M cacodylate buffer containing 7% sucrose, postfixed with 1% osmium tetraoxide in 0.15 M posphate buffer for 1 hr at 4°C, dehydrated in a graded ethanol series, and embedded in LR white resin (London Kes in Company Ltd, Berkshire, UK), which was then incubated at 55°C for 48 hr. Ultrathin sections were placed on Formvar-coated nickel grids and treated with 1% meta- periodic acid for 10 min, followed by 1% BSA in PBS for 1 hr. The primary antibody used was the polyclonal antiserum against porcine ACTH (1: 200). Sections were incubated overnight with this antigen at 4°C, washed with PBS, treated with gold-labeled (10 nm) secondary antibody (1: 20; British BioCell International, Cardiff, UK) for 1 hr, washed, and observed with a Hitachi H700H electron microscope operated at 100 kV. Control staining was performed by treating sections with the primary antiserum (1: 200, 1 ml) preabsorbed with antigen (100 μg) as described above.

RESULTS

A considerable number of the cells scattered around the tubular structure of the dorsal strand were immunoreactive with the antiserum against ACTH (Figs. 1 and 2A). A few cells in the cerebral ganglion were also immunopositive with the antiserum (data not shown). However, no cells in the neural gland were ACTH-immunopositive (Fig. 1). Staining of adjacent sections with the antiserum against PRL revealed that the ACTH-immunopositive cells are different from the PRL-immunopositive ones (Fig. 2B). The immunoreaction was prevented by preabsorption of the anti-ACTH (Fig. 2C) or the anti-PRL (Fig. 2D) with the appropriate antigen.

Fig. 1

Immunocytochemical staining of the dorsal strand with anti-porcine ACTH serum. The ACTH-imunoreactive cells are distributed among the tubular structures of the dorsal strand. Empty spaces within and around the tissues of the dorsal strand constitute the dorsal blood sinus. ds, dorsal strand, ng, neural gland. Bar: 100 μm

Fig. 2

Four adjacent sections stained with anti-ACTH (A), anti-PRL (B), anti-ACTH preabsorbed with antigen (C) and anti-PRL preabsorbed with antigen (D). Equivalent cells in “A” and “B” are indicated by black (ACTH- immunoreactive cells) and white (PRL- immunoreactive cells) arrowheads. Bar: 10 μm

Immunoelectron microscopic study revealed that the gold particles were mostly localized in the secretory granules with diameters of about 300–500 nm (Fig. 3A, B). When the antiserum preabsorbed with ACTH was applied, the gold particles on the secretory granules were reduced in number to the back ground level (data not shown).

Fig. 3

Immunoelectron microscopy of dorsal strand. (A) Immunoelectron micrograph of ACTH-immunoreactive cells distributed in the dorsal strand. Bar: 1 μm. (B) A higher magnification of the region indicated by the rectangle in “A”. Bar: 0.5 μm. Gold particles are localized over secretory granules that measure about 300–500 nm in diameter.

DISCUSSION

In a previous communication, we reported that some of the cells in the dorsal strand and the cerebral ganglion contained a PRL-like immunoreactive material within their secretory granules (Terakado et al., 1997). In the present experiment, ACTH-like immunoreactivity was also demonstrated in a considerable number of cells in the dorsal strand and in a few cells in the cerebral ganglion. The preservation of membranous structures and cell organella of our preparations for immunoelectron microscopic study was rather poor. This was due to the use of LR white resin for embedding of the tissue, which is known to preserve immunoreactivity. However, it was obvious that the immunoreactivity resided within the secretory granules. Moreover, it was apparent that ACTH-like substance and PRL-like substance were localized in different cells. Of note, the ACTH-like substance was contained within the granules with a diameter of approximately 300–500 nm, which are the largest among the granules found in the cerebral ganglion and the dorsal strand. On the other hand, the PRL-like substance was detected in the granules of about 100–250 nm in diameter (Terakado et al., 1997).

Earlier studies by Pestarino (1984, 1985a, b) showed the presence of ACTH-like immunoreactive substance and PRL-like immunoreactive substance in the neural gland of another ascidian, Styela plicata. Although the existence of these substances in the cerebral ganglion of the same species was also reported by the same investigator (Pestarino, 1983, 1988), the occurrence of pituitary hormone-like immunoreactive substances in the dorsal strand had never been pointed out. On the contrary, we have observed the presence of neither secretory granules nor of ACTH-like and PRL-like immunoreactivities in the neural gland of H. roretzi, whereas a considerable number of the cells in the dorsal strand of this species did contain these PRL-like and ACTH-like substances. At moment it is not clear whether the discrepancy between these two species of ascidians in terms of localization of ACTH-like and PRL-like immunoreactive cells in the neural complex is due to the species difference, difference in some physiological conditions of the specimens when examined, difference in properties of antisera used in each experiment or some other reason.

More recently, Pestarino and his group provided an evidence that some of the cerebral ganglion cells of S. plicata expressed the mRNA of a POMC-like molecule (Masini et al., 1998). In vertebrates, the pituitary POMC molecule is cleaved by prohormone convertases to generate bioactive peptides such as ACTH, α-melanophore-stimulating hormone (α-MSH) and β-endorphin. In fact, the occurrence of immunoreactivities indicating the presence of POMC-related peptides such as ACTH (Fritsch et al., 1982, Georges and Dubois 1979, Pestarino 1988) α-MSH (Pestarino, 1988) and β-endorphin (Pestarino, 1985c) in the cerebral ganglion of two species of ascidians, Ciona intestinalis and S. plicata has been reported. The prohormone convertases that generate the POMC-related peptides are known to be PC1 and PC2 (Benjannet et al., 1991; Thomas et al., 1991). Very recently we recognized that some cells in the cerebral ganglion as well as in the dorsal strand possessed PC1 and PC2-like substances (Kawahara et al., 2001).

On the other hand, immunoreactive GnRH has been localized in the dorsal strand and the cerebral ganglion of H. roretzi (Terakado and Ogawa, 1995). Subsequently, two forms of GnRH have been isolated from the neural complex of an ascidian, Chelyosoma productum and one of them has been localized in the dorsal strand (Powell et al., 1996).

In view of these results, it is highly probable that the cerebral ganglion and dorsal strand of ascidians contain a cell population equivalent to the hypothalamic and/or pituitary cells in vertebrates.

Acknowledgments

This work was supported by research grants from Waseda University, Asahi Glass Research Foundation, Uehara Memorial Foundation, and the Ministry of Education, Science, and Culture of Japan to S.K. and by a Sasakawa Scientific Research Grant from the Japan Science Society to G.K. We thank Dr. S. Tanaka at Shizuoka University for the gift of anti-ACTH serum.

REFERENCES

1.

S. Benjannet, N. Rondeau, R. Day, M. Chretien, and N. G. Seidah . 1991. PC1 and PC2 are proprotein convertases capable of cleaving proopiomelanocortin at distinct pairs of basic residues. Proc Natl Acad Sci USA 88:3564–3568. Google Scholar

2.

G. F. Couly and N. M. Le Douarin . 1985. Mapping of the early neural primordium in quail-chick chimeras. I. Developmental relationships between placodes, facial ectoderm and prosencephalon. Dev Biol 110:422–439. Google Scholar

3.

G. F. Couly and N. M. Le Douarin . 1987. Mapping of the early neural primordium in quail-chick chimeras.II. The prosencephalic neural plate and neural folds: Implications for the genesis of cephalic congenital abnormalities. Dev Biol 120:198–214. Google Scholar

4.

J. M. Dodd and M. H. I. Dodd . 1966. An experimental investigation of the supposed pituitary affinities of the ascidian neural complex. In “Some contemporary studies in marine science”. Ed by H. Barnes Allen & Unwin. London. pp. 233–252. Google Scholar

5.

G. W. Eagleson, B. L. Jenks, and A. P. van Overbeeke . 1986. The pituitary adrenocorticotropes originate from neural ridge tissue in Xenopus laevis. J Embryo Exp Morphol 95:1–4. Google Scholar

6.

H. A. R. Fritsch, S. Van Noorden, and A. G. E. Pearse . 1982. Gastro-intestinal and neurohormonal peptides in the alimentary tract and cerebral complex of Ciona intestinalis (Ascidiaceae). Cell Tissue Res 223:369–402. Google Scholar

7.

D. Georges and M. P. Dubois . 1979. Immunological evidence for an ACTH-like antigen in the nervous ganglion of a protochordate Ciona intestinalis (Ascidiacea). Arch Anat Microsc Morph Exp 68:121–125. Google Scholar

8.

D. Georges and M. P. Dubois . 1985. Presence of vertebrate-like hormones in the nervous system of a tunicate, Ciona intestinalis. In “Current trends in comparative endocrinology”. Ed by B. Lofts and W. H. Holmes . University Press. Hong Kong. pp. 54–57. Google Scholar

9.

G. Kawahara, K. Terakado, S. Tanaka, and S. Kikuyama . 2001. Existence of PC1- and PC2-like immunoreactive substances in the ascidian neural complex. Abstracts for 14th International Congress of Comparative Endocrinology. Sorrento. p. 63. Google Scholar

10.

K. Kawamura and S. Kikuyama . 1992. Evidence that hypophysis and hypothalamus constitute a single entity from the primary stage of histogenesis. Development 115:1–9. Google Scholar

11.

T. Kouki, H. Imai, K. Aoto, K. Eto, K. Kawamura, and S. Kikuyama . 2001. Developmental origin of the rat adenohypophysis prior to the formation of Rathke's pouch. Development 128:959–963. Google Scholar

12.

M. A. Masini, M. Sturla, A. Gallinelli, S. Candiani, F. Facchinetti, and M. Pestarino . 1998. Expression of proopimelanocortin (POMC) in the cerebral ganglion and ovary of a protochordate. Peptides 197:1177–1181. Google Scholar

13.

M. Pestarino 1983. Prolactinergic neurons in a protochordate. Cell Tissue Res 233:471–474. Google Scholar

14.

M. Pestarino 1984. Immunocytochemical demonstration of prolactin-like activity in the neural gland of the ascidian Styela plicata. Gen Comp Endocrinol 54:444–449. Google Scholar

15.

M. Pestarino 1985a. A pituitary-like role of the neural gland of an ascidian. Gen Comp Endocrinol 60:293–297. Google Scholar

16.

M. Pestarino 1985b. Localization of α-MSH-like immunoreactive cells in the neural gland of the ascidian Styela plicata. Cell Tissue Res 240:497–500. Google Scholar

17.

M. Pestarino 1985c. Occurrence of β-endorphin-like immunoreactive cells in the neural complex of a protochordate. Cell Mol Biol 31:27–31. Google Scholar

18.

M. Pestarino 1988. Occurrence of melanotropin-and corticotropin-like material in the cerebral ganglion of a protochordate. Neurosci Lett 87:210–214. Google Scholar

19.

J. F. Powell, S. M. Reska-Skinner, M. O. Prakash, W. H. Fischer, M. Park, J. E. Rivier, A. G. Craig, G. O. Mackie, and N. M. Sherwood . 1996. Two new forms of gonadotropin-releasing hormone in a protochordate and the evolutionary implications. Proc Natl Acad Sci USA 93:10461–10464. Google Scholar

20.

S. Tanaka and K. Kurosumi . 1986. Differential subcellular localization of ACTH and alpha-MSH in corticotropes of the rat anterior pituitary. Cell Tissue Res 243:229–238. Google Scholar

21.

K. Terakado and M. Ogawa . 1995. Secretory cells scattered along the dorsal strand of ascidians. 3. Gonadotropic hormone-positive cells. In “Proceeding of the Japan Society for Comparative Endocrinology”Ed by Y. Sasayama and N. Suzuki . Hayashi Kobo. Tokyo. No 10. p. 30. Google Scholar

22.

K. Terakado, M. Ogawa, K. Inoue, K. Yamamoto, and S. Kikuyama . 1997. Prolactin-like immunoreactivity in the granules of neural complex cells in the ascidian Halocynthia roretzi. Cell Tissue Res 289:63–71. Google Scholar

23.

L. Thomas, R. Leduc, B. A. Thorne, S. P. Smeekens, D. F. Steiner, and G. Thomas . 1991. Kex2-like endoproteases PC2 and PC3 accurately cleave a model prohormone in mammalian cells: evidence for a common core of neuroendocrine processing enzymes. Proc Natl Acad Sci USA 88:5297–5301. Google Scholar

24.

K. Yamamoto and S. Kikuyama . 1982. Radioimmunoassay of prolactin in plasma of bullfrog tadpoles. Endocrinol Jpn 29:159–167. Google Scholar

Citation Download Citation

Genri Kawahara, Kiyoshi Terakado, Toshio Sekiguchi, Kinji Inoue, and Sakae Kikuyama "Adrenocorticotropin-Like Immunoreactivity in the Granules of Neural Complex Cells of the Ascidian Halocynthia roretzi," Zoological Science 19(9), 1061-1065, (1 September 2002). https://doi.org/10.2108/zsj.19.1061

Received: 4 June 2002; Accepted: 1 July 2002; Published: 1 September 2002

JOURNAL ARTICLE
5 PAGES

DOWNLOAD PAPER + SAVE TO MY LIBRARY