Jm. Grondona et al., ANALYSIS OF THE SECRETORY GLYCOPROTEINS OF THE SUBCOMMISSURAL ORGAN OF THE DOGFISH (SCYLIORHINUS-CANICULA), Molecular brain research, 26(1-2), 1994, pp. 299-308
The subcomissural organ (SCO) is an ancient and conserved brain gland
secreting glycoproteins into the cerebrospinal fluid which condense to
form Reissner's fiber (RF). The SCO of an elasmobranch species, the d
ogfish Scyliorhimus canicula, was investigated applying morphological
and biochemical methods. The SCO of 34 dogfishes were processed for th
e following techniques: (1) conventional transmission electron microsc
opy; (2) light and electron microscopy lectin histochemistry (Concanav
alin A, Con A; wheat germ agglutinin, WGA; Limax flavus agglutinin, LF
A); (3) light and electron microscopy immunocytochemistry using antise
ra raised against the glycoproteins of the bovine RF (anti-bovine RF),
and the secretory material of the dogfish SCO (anti-dogfish SCO). The
former reacts with the SCO of virtually all vertebrate species [19] (
conserved epitopes); the latter reacts only with the SCO of elasmobran
chs [Cell Tissue Res., 276 (1994) 515-522] (class-specific epitopes).
At the light microscopic level both antisera immunoreacted selectively
with the SCO and RF; no other structure of the central nervous system
was reactive. Within the SCO the binding sites for WGA (affinity = gl
ucosamine, sialic acid) and LFA (affinity = sialic acid) displayed the
same density and intracellular distribution. At the ultrastructural l
evel two types of granules were distinguished. Type I granules (200-40
0 nm) were numerous, reacted with both antisera, bound WGA but not Con
A. Type II granules (0.8-1.8 mu m) reacted with the anti-bovine RF se
rum but not with the anti-dogfish SCO serum, bound Con A and WGA. The
content of dilated cisternae of the rough endoplasmic reticulum reacte
d with both antisera and bound Con A; it did not bind WGA. The SCOs of
4500 dogfishes were extracted in ammonium bicarbonate. This extract w
as used for SDS-PAGE and blotting. Blots were processed for immunolabe
ling using anti-bovine RF and anti-dogfish SCO sera, and for lectin bi
nding (Con A, WGA and LFA). The anti-bovine RF revealed four compounds
with apparent molecular weights of 750, 380, 145 and 35 kDa. The two
former also reacted with the anti-dogfish SCO serum and bound Con A. O
nly the 380 kDa compound bound WGA and LFA. The findings indicate that
both the conserved and the class-specific epitopes are part of the sa
me compounds (780, 380 kDa), which would be stored in type I granules.
The lectin binding properties of these compounds point to the 780 kDa
compound as a precursor form and the 380 kDa polypeptide as a process
ed form.