Minoru Amano

Regulation of protein synthesis by estradiol 17β, dexamethasone and insulin in primary cultured Xenopus hepatocytes☆

Changes in the protein synthesis of Xenopus hepatocytes caused by insulin, estradiol-17 beta (estradiol) and dexamethasone were studied by using a primary culture in serum-free medium. All of these hormones stimulated the synthesis of secretory and intracellular proteins. Dexamethasone induced or stimulated the synthesis of many proteins (though limited in number), whereas estradiol induced or stimulated relatively few proteins, including the yolk precursor protein vitellogenin. The majority of these proteins differed in molecular weight and/or isoelectric point. When hepatocytes were treated with both steroids, most of the proteins were synthesized at the rates expected from the single treatment of the respective steroids. Thus, each steroid selectively stimulated the synthesis of its specific proteins. However, exceptional proteins were observed, whose syntheses were stimulated only by double treatment. In contrast, insulin seemed to cause an overall increase in individual secretory protein synthesis.

Quantitative Analysis of Protein Synthesis Altered by Estrogen in Cultured Xenopus Liver Parenchymal Cell

Using the primary culture system of male Xenopus laevis hepatocytes consisting of more than 95% parenchymal cells, the effect of estradiol‐17 β (10−6M) on protein synthesis was quantitatively analyzed by 3H‐leucine incorporation kinetics and the estimation of specific radioactivity of newly synthesized secretory protein. The cells in a well defined culture revealed high plating efficiency and very low DNA synthetic activity. The cultured cells could synthesize several secretory proteins containing serum albumin. The pattern of secreted proteins in SDS‐polyacrylamide gel electrophoresis (SDS‐PAGE) did not alter with culture time but secretion rate of protein increased for 7 days, starting on the third day following inoculation. Estradiol added to the culture media extensively induced the synthesis of yolk precursor protein vitellogenin which accounted for 40–50% of the overall secretory protein synthesis and 20–30% of the total protein synthesis on day 7 of estradiol treatment. Ultimately, the total protein synthesis and secretory protein synthesis were stimulated 1.2–1.3 fold and 2.0–2.2 fold, respectively, over those of the control cells cultured in the absence of estradiol. These results indicated that the stimulation of protein synthesis was largely due to vitellogenin production. Such an estradiol‐dependent stimulation of protein synthesis was also detected in the low molecular weight protein(s). On the other hand, albumin synthesis was evidently reduced by estradiol. Thus, estradiol had two different effects on protein synthesis.

A change of the hepatocyte population is responsible for the progressive increase of vitellogenin synthetic capacity at and after metamorphosis of Xenopus laevis

Synthesis of the egg yolk precursor protein, vitellogenin, can be induced in adult, but not in larval, amphibian hepatocytes by estrogen treatment. The transition process for this inducibility of hepatocytes during development of Xenopus laevis was examined, using primary cultures of hepatocytes. This was found to occur at about the metamorphic climax of stage 62, although the level of vitellogenin production was very limited at this stage. This low level seemed due neither to insufficient estradiol-17 beta nor to high estrogen-degrading activity. The level of synthesis gradually increased following metamorphosis. Immunohistochemical analysis showed that fewer than 5% of the hepatocytes at stage 62 could be stained with antivitellogenin antibody and that the stained cell fraction subsequently increased gradually for several months after metamorphosis. These findings indicate that adult-type cells capable of synthesizing vitellogenin appear at metamorphosis and then expand their population in the liver during postmetamorphic maturation.

Scleral fibroblasts of the chick embryo proliferate by an autocrine mechanism in protein-free primary cultures: Differential secretion of growth factors depending on the growth state

Scleral fibroblasts of the chick embryo in primary culture proliferated in a protein-free medium. Conditioned medium (CdM) from the culture contained plural growth-promoting factors, which were active to the same cell type. The activity of one of the growth-promoting factors (SAF-I) was heat-resistant and the rest (SAF-II) were heat-sensitive. SAF-I accumulated in the CdM only during the growing phase; on the other hand, SAF-II accumulated in the CdM during the stationary phase. SAF-I showed the same time course of DNA synthesis-promoting activity as human PDGF. However, the activity of the SAF-I was not neutralized by anti-human PDGF. On the other hand, a part of the SAF-II (SAF-II a) showed a strong affinity for heparin.

Analysis of the Formation of the Animal- Vegetal Axis during Xenopus Oogenesis Using Monoclonal Antibodies

Maternally accumulated materials in Xenopus oocytes, in particular mRNAs and proteins, are considered to participate in the determination of the developmental specification of embryonic cells. In this study, a large number of monoclonal antibodies was raised against bulk oocyte antigens to examine patterns of intracellular distribution of oocyte proteins. Immunohistochemical experiments with mature oocytes showed that there are five different patterns of distribution of oocyte proteins, with enrichment on the animal side (type A1, and A2 ptoteins), vegetal side (type V1 and V2 proteins), and in the peripheral cytoplasm (type P proteins). Clear localization of type A and V antigen proteins occurred at Dumonts stages IV‐VI. However, at the preceding stages, the distributions of these antigen proteins appeared to be homogeneous. By contrast, the pattern of distribution of type P protenis did not change markedly throughout oogenesis. The presence of type A and type V antigen proteins reflected the animal‐vegetal axis in the cytoplasm of the mature oocyte. Furthermore, there were two boundaries of the distributions of proteins at the equatorial region, excluding or including the cytoplasm around the germinal vesicle. Thus, the cytoplasm of mature oocytes was multilayered with respect to the different proteins distributed along the animal‐vegetal axis.

Purification of an autocrine growth factor in conditioned medium obtained from primary cultures of scleral fibroblasts of the chick embryo

Scleral fibroblasts of the chick embryo were found to secrete autocrine growth factors. One of the factors was purified from conditioned medium collected from growing-phase cultures of these cells by DEAE-Sepharose column chromatography and following non-denaturing polyacrylamide gel electrophoresis. The specific activity was increased 1100-fold by this purification. The chromatographically purified growth factor was still active after incubation at 95 degrees C, at pH 10 or pH 3, or with glycosidase H, but inactive after incubation with dithiothreitol or trypsin. An active protein having a molecular weight of 32 kDa was found to be the major component of the final preparation.

In vitro growth of adult amphibian (Xenopus laevis) hepatocytes and characterization of hepatocyte-proliferating activity in homologous serum.

Adult frog (Xenopus laevis) hepatocytes were found to proliferate in a culture medium containing adult homologous serum. Insulin and dexamethasone were required for a net proliferation of hepatocytes. Dose-response analysis showed that a low concentration of serum (greater than or equal to 0.5%) was enough to induce DNA synthesis and mitosis, but a higher concentration (5%) caused certain necrotic changes. Under optimal conditions, there was a two- to threefold increase in nuclei per culture 10 days after serum treatment. Heterologous sera (fetal bovine, calf and chick) showed less proliferative activity. Based on our results, hepatocyte-proliferating activity in adult frog serum is considered to be heat-unstable and acidic protein(s). Thus, adult frog serum may contain hepatopoietin possibly different from well-known growth factors.