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1.
本文研究河蚌外套膜组织培养细胞分泌珍珠质的药理作用。组织培养后的培养液,能缩短小白鼠出血时间。用组织培养后的培养液及组织块水解液,对大鼠离体子宫及蟾蜍离体心脏收缩有增强作用,对兔离体小肠有抑制作用。这些药理作用与培养液中牛磺酸含量变化一致。实验结果表明,河蚌分泌珍珠质的细胞,在离体人工培养条件下,能旺盛地分泌珍珠质,分泌的珍珠质具有天然珍珠相同的一些药理作用。  相似文献   

2.
河蚌培养组织的几种生化成分分析   总被引:1,自引:0,他引:1  
本文分析测定了三角帆蚌,褶纹冠蚌和背角无齿蚌外套膜培养组织及其培养液中的氨基酸,牛磺酸及钙含量。在珍蛛中含量较高的丙的氨酸和甘氨酸分别增加541%和91%。三种蚌在培养中牛磺酸含量增加5.78%到3倍,培养组织的钙含量增加1倍左右。同时测定了培养组织的碱性磷酸酶活性,培养组织与河蚌外套膜具有相近的比活及相对酶活。结果表明,河蚌外套膜在离体培养条件下,也具有分泌珍珠质的能力。  相似文献   

3.
褶纹冠蚌外套膜组织培养的分泌物的偏光显微镜观察   总被引:3,自引:0,他引:3  
以淡水育珠贝中珍珠形成较快的褶纹冠蚌为材料,用相差显微镜观察组织培养的外套膜的分泌物的形成和变化,用偏光显微镜观察分泌物的双折射现象,并与活体外套膜的分泌物、贝壳的角质层、棱柱层、珍珠层的双折射现象进行比较。结果表明;离体培养的外套膜细胞不仅能产生活体细胞相同的分泌物,而且分泌物还能在培养过程中形成结晶,并逐渐生长。发现外套膜的不同部位分区培养所形成的分泌物的性状与结晶性质和活体有一致性,表明组织培养的外套膜小片具有贝体原来的组织结构、分化特征和分泌功能。  相似文献   

4.
不同pH值对三角帆蚌珍珠质分泌的影响   总被引:14,自引:0,他引:14  
邱安东  石安静 《动物学报》1999,45(4):361-370
运用多种组织化学方法和透射电镜技术,研究了5种pH水环境(pH5、6、7、8、9)对三角帆砷外套膜珍珠质分泌的影响机制,结果表明,在中性水环境中,贝体能积极地从外界水环境中吸收钙,并能旺盛地合成和分泌贝壳珍珠层及珍珠有机基质前体物质,持续的酸性水环境导致贝体的钙严重丢失,并引起珍珠质分泌细胞对有机基质前体物质的合成和分泌能力减弱,持续的碱性水环境虽能导致贝体对钙的积累,但珍珠质分泌细胞合成和分泌珍  相似文献   

5.
褶纹冠蚌外套膜组织培养的分泌物的偏光显微镜…   总被引:3,自引:0,他引:3  
以淡水育珠贝中珍珠形成较快的褶纹冠蚌为材料,用相差显微镜观察组织培养的外套膜的分泌物的形成和变化,用偏光显微镜观察分泌物的双折射现象,并与活体外套膜的分泌物、贝壳的角质层、棱柱层、珍珠层的双折射现象进行比较。结果表明:离体培养的外套膜细胞不仅能产生活体细胞相同的分泌物,而且分泌物还能在培养过程中形成结晶,并逐渐生长。发现外套膜的不同部位分区培养所形成的分泌物的性状与结晶性质和活体有一致性,表明组织  相似文献   

6.
作者用扫描电镜及相差显微镜,对椭圆背角无齿蚌外套膜组织培养与未培养细胞的分泌活动进行了研究,观察到两者的分泌活动都是十分旺盛的。培养细胞有局部分泌和顶浆分泌。细胞分泌形态观察到三种:(1)分泌端形成由膜包裹的突起,突起逐渐伸长,基部变成细颈,最后脱离细胞成为分泌泡(局部分泌);(2)细胞端部伸出长足,将分泌物排到较远处分泌后,长足缩回恢复原状;(3)分泌端伸出很多细枝,分泌物随后如液流式涌出细胞(顶浆分泌)。取外套膜色线边组织为材料,培养后在组织块和细胞上有角质素(与贝壳最外层相似)类的茶褐色结晶和无定形分泌物形成;用去掉色线边的外表皮组织块培养,则有珍珠(与贝壳最内层相似)状的白色和淡黄色结晶生成。表明了细胞在适宜的条件下培养,所形成的分泌物的性质可能与活体相同。因此大批量培养细胞可能得到人们希望获得的细胞产物。  相似文献   

7.
背角无齿蚌珍珠囊形成过程中钙代谢的初步研究   总被引:2,自引:0,他引:2  
本文采用同位素活体标记、人工育珠、普通石蜡切片和放射自显影的方法,对一种淡水育珠河蚌──背角无齿蚌珍珠囊形成过程中的钙代谢途径进行了研究,结果表明,由植入小片带入的钙在珍珠囊形成的过程中,主要代谢途径是:(1)随小片细胞脱落而进入游走细胞;(2)从小片进入初生珍珠囊,初生珍珠囊脱落后进入游走细胞;(3)从小片进入育珠蚌结缔组织,其中一部分再进入育珠蚌表皮,随粘液和壳质分泌;另一部分则进入次生珍珠囊表皮,分泌成为珍珠质的组成部分。实验结果说明了小片中的钙要参与育珠蚌组织的钙代谢,小片的质量对珍珠形成有重要的作用。  相似文献   

8.
褶纹冠蚌珍珠囊发育的研究   总被引:10,自引:1,他引:9  
以褶纹冠蚌(Cristaria plicata Leach)为实验对象,应用光学显微技术和扫描电子显微技术研究珍珠囊的发育,结果表明在水温16℃左右时约需30d形成具有单层上皮细胞的珍珠囊,6个月后稳定分泌珍珠质。构成珍珠囊的上皮细胞从高柱状逐渐变成扁平状或立方形,细胞的碳酸酐酶污性也日益增强。大部分移植细胞小片的结缔组织与母蚌的结缔组织共同成层排列在珍珠囊腔外围。游走细胞在珍珠囊的早期发育阶段十分活跃。本文还阐明了珍珠囊液是存在于上皮细胞与珍珠表面之间的一薄层流体状物质。碳酸钙结晶的核化(nucleation)和初期生长都发生在珍珠囊液中。  相似文献   

9.
褶纹冠蚌光珠与骨珠珍珠囊差异的研究   总被引:7,自引:0,他引:7  
运用多种组织化学方法和电镜技术研究了褶纹冠蚌光珠和骨珠珍珠囊表皮细胞的形态结构、分泌物性质和功能等方面的差异。结果表明:骨珠珍珠囊表皮细胞合成和分泌珍珠前体物质的能力较光珠的强,故骨珠的形成速度比光珠快;光珠和骨珠珍珠囊表皮细胞合成和分泌的蛋白质的差异决定了光珠和骨珠的形成;光珠和骨珠珍珠囊表皮细胞的形态结构特征差异可作为检验和预测人工培育珍珠质量的细胞学标准。  相似文献   

10.
以圆前角无齿蚌为材料,采用外套膜小片的异体移植与加入血细胞的体外培养,研究了血细胞在体风,唯物 修复及珍珠囊构建中的功能。结果表明人工育珠手术后的损伤修复中,血细胞有形成无颗粒细胞层修复伤口、6诱导表皮细胞迁移和再生并形成珍珠囊的功能,而在体外的组织培养中加入血细胞比不加入血细胞的对照组,能更快地诱导上皮细胞迁移和再生,在整个伤面形成2覆盖层,即形成类似珍珠囊结构。本文首次在国内、外报道了用细胞培  相似文献   

11.
1. The rate of fatty acid synthesis by mammary explants from rabbits pregnant for 16 days or from rabbits pseudopregnant for 11 days was stimulated up to 15-fold by culturing for 2-4 days with prolactin. This treatment initiated the predominant synthesis of C(8:0) and C(10:0) fatty acids, which are characteristic of rabbit milk. 2. Inclusion of insulin in the culture medium increased the rate of synthesis of these medium-chain fatty acids. By contrast the inclusion of corticosterone led to the predominant synthesis of long-chain fatty acids. When explants were cultured for 2-4 days with insulin, corticosterone and prolactin, the rate of fatty acid synthesis increased up to 42-fold, but both medium- and long-chain fatty acids were synthesized. 3. These results show that the stimulus to mammary-gland lipogenesis and the initiation of synthesis of medium-chain fatty acids observed between days 16 and 23 of pregnancy in the rabbit can be simulated in vitro by prolactin alone. 4. When mammary explants from rabbits pregnant for 23 days were cultured for 2 days with insulin, corticosterone and prolactin, the rate of fatty acid synthesis increased fivefold, but there was a preferential synthesis of long-chain fatty acids. Culture with prolactin alone had little effect on the rate or pattern of fatty acids synthesized. 5. The results are compared with findings in vivo on the control of lipogenesis in the rabbit mammary gland, and are contrasted with the known effects of hormones in vitro on the mammary gland of the mid-pregnant mouse.  相似文献   

12.
Free amino acids and amines in leaf explants of Nicotiana tabacum cultivated in vitro on media inducing rhizogenesis or caulogenesis.
Foliar explants of Nicotiana tabacum cv. Xanthi n.c. were cultivated on three different media: (1) a basal medium without hormone, so that no differentiation occurred in the explants; (2) with auxin added; and (3) with auxin plus cytokinin added, where the additions (2) and (3) promote rhizogenesis and caulogenesis, respectively. The content of free amino acids and amines of the three kinds of explants were investigated. In the two media lacking cytokinin, the explants contained great amounts of five amino acids (asparagine, glutamine, proline, glutamic acid and histidine) and of one aromatic amine, tyramine. In the cytokinin containing medium, only two amines accumulated in the explants: one aliphatic polyamine (putrescine) and one aromatic amine (phenethylamine). The increase in amino acids began immediately on the first days of culture. It was related neither to a more active proteolysis nor to the breaking of the correlations from the mother plant. It was induced by the addition of nutritional elements into the medium. On the other hand, the accumulation of aromatic amines occurred after a few days of culture and was transitory. A decrease was observed after the first emergence of new organs. The relation between the accumulations of these aromatic compounds and formation of roots or shoots is discussed.  相似文献   

13.
The media, in which a butterfly cell line (Px 58), derived from pharate adult ovaries of Papilio xuthus cultured for 8 days, were analysed to examine the changes in free amino acids in the medium during cultivation. Beta-alanine, arginine, glycine, histidine, lysine, phenylalanine, proline, serine, and tryptophan did not change markedly. Asparagine, aspartic acid, cystine, glutamine, isoleucine, leucine, methionine, threonine, tyrosine, and valine decreased to some extent with culturing. Alpha-alanine increased markedly, and glutamic acid did so to a lesser extent. Requirements of amino acids by the cell line were examined by deleting amino acids one at a time. Deletion of alpha-alanine, beta-alanine, asparagine, glutamic acid, glycine, and phenylalanine did not cause deterioration of the cell. These amino acids were thought to be non-essential or required only a little. Deletion of other amino acids impaired the cell growth severely. These amino acids would appear to be essential for growth of the Px 58 cell line.  相似文献   

14.
The fatty acid composition of cultured Friend erythroleukemia cells was modified by supplementation of the medium with oleic or linoleic acid. There was a 30% reduction in saturated and a 35% reduction in polyunsaturated fatty acids in microsomal phospholipids when the cells were grown in media supplemented with oleic acid, and a 3-fold increase in polyunsaturated fatty acids when the cells were grown in linoleic acid-supplemented media. Electron-spin resonance studies with the 5-nitroxystearate probe demonstrated that there was no appreciable change in microsomal lipid mobility as measured by the order parameters. In contrast, changes in lipid mobility were detected with the spin-label probe when microsomes were first isolated from Friend erythroleukemia cells and subsequently modified by incubation with liposomes composed of either dioleoyl- or dilinoleoylphosphatidylcholine plus bovine liver phospholipid-exchange protein. The fatty acid compositional changes produced in these microsomes were similar to those obtained when the intact cells were grown in media containing supplemental fatty acids. These findings indicate that the lipid mobility of Friend cell microsomes can be altered by phospholipid replacements in vitro, but that this does not occur when similar microsomal fatty acid modifications are produced during culture of the intact cell.  相似文献   

15.
在生根焙养基中加入0.5或2.0ppm PP_333,明显地减少了苹果离体新梢的鲜重和干重、叶片鲜重和叶面积,增加了比叶重、根的鲜重和干重及根梢鲜重和干重比,并促进了根的形成。PP_333对单位叶重量的叶绿素含最没有影响,而增加了单位叶面积的叶绿素含量。经PP_333处理后,叶片中的淀粉含量、过氧化物酶活性、蛋白质和游离氨基酸的含量均明显离于对照,可溶性糖与对照差异不明显。  相似文献   

16.
Total protein was determined for cells of Aphanothece halophytica Fremy harvested during early log, mid-log and linear growth phases in media containing 1, 2, and 3 M NaCl. Cells grown in medium containing 1 M NaCl showed a progressive increase in protein content up to a maximum of 76% of dry weight (linear phase). Total protein also increased in cells grown in 2 M NaCl. medium (56.5–72.0%). Cells grown in 3 M NaCl medium showed a progressive decrease in total protein (59.9–43%). Although amounts of protein varied, the percentages of the respective amino acids of hydrolyzed bulk protein were consistent to within 1% for linear phase cells grown in 1, 2, and 3 M NaCl cultures. Percentages of acidic amino acids were 2.3–2.6 times greater than those of the basic amino acids. The amino acid composition of phycocyanin was similar to that of bulk protein. Free amino acids varied with both age of the culture and the concentration of NaCl. The high quantity and quality of the protein observed suggest that A. halophytica might be a useful food organism.  相似文献   

17.
Cylinders of carrot taproot secondary phloem were cultured on one of four media: 1) 2% sucrose + 1% agar (SA); 2) Heller's basal medium (NA); 3) NA + 10-5 g/liter 2,4-D (H4); and 4) NA + H4 + 15% coconut milk (HW). Samples were taken from the cultured explants at 3-day intervals. A morphological study of the cultured explants revealed no differences between callus-initiating explants (cultured on HW medium) and noncallus-initiating explants (cultured on SA, NA, and H4 media) within the first 3 days of culture. All explants exhibited a typical wound response. Cell division ceased in the NA and SA explants after the sixth day in culture. Extensive cell division occurred in the subsurface layer of dividing cells in the HW explants and resulted in the formation of callus by the ninth day in culture. Histochemical staining revealed that the activity of NAD diaphorase, succinic dehydrogenase, and cytochrome oxidase were closely correlated with the wound response and with callus initiation in the cultured explants. The activity of these enzymes was high in the layer of dividing cells of all explants after 3 days of culture, but with longer periods of culture the activity of these enzymes was closely correlated with the extent of cell division. Acid phosphatase activity was associated with the dividing cell layers of all explants, but comparatively little acid phosphatase activity was observed in the NA, SA, and H4 explants as compared to the HW explants, and acid phosphatase was strongly correlated with callus initiation by the HW explants. Using the nitroso reaction, “catechol tannins” were found in the surface layers of the NA, SA, and H4 explants, while no nitroso-reaction-positive substances were detected in the HW explants during the period of callus initiation.  相似文献   

18.
Long-term supplementation of branched-chain amino acids (BCAA) improves hypoalbuminemia in patients with cirrhosis. Our previous findings have suggested that the binding of polypyrimidine-tract-binding protein (PTB) to rat albumin mRNA attenuates its translation. The aim of the present study was to investigate the role of PTB in the regulation of albumin synthesis by BCAA in human hepatoma cells. HepG2 cells were cultured in a medium containing no amino acids (AA-free medium), a medium containing only 1 amino acid (a BCAA: valine, leucine or isoleucine) or a medium containing all 20 amino acids (AA-complete medium). HepG2 cells cultured in AA-complete medium secreted much more albumin than cells cultured in AA-free medium, with no difference in albumin mRNA levels. In cells cultured in AA-free medium, nuclear export of PTB was observed, and the level of the albumin mRNA-PTB complex was greater than in cells cultured in AA-complete medium. Addition of amino acids stimulated nuclear import of PTB. However, addition of amino acids with rapamycin inhibited the nuclear import of PTB. The addition of leucine, but not of valine or isoleucine, to AA-free medium increased albumin secretion and stimulated the nuclear import of PTB. These data indicate that the mammalian target of rapamycin is involved in the regulation of PTB localization and that leucine promotes albumin synthesis by inhibiting the formation of the albumin mRNA-PTB complex.  相似文献   

19.
Summary A previous finding that insulin cells do not survive or differentiate in explants of embryonic avian pancreas cultured in collagen gel with a serum-containing medium has provided a model system for identification of conditions favorable for development of these cells. To this end, we here modify the substrate and the medium. The epithelial component of dorsal pancreatic buds of 5-d chick embryos was cultured for 7 d on Matrigel in serum-containing and in serum-free medium, the latter incorporating insulin, transferrin, and selenium, Endocrine cell types were distinguished by immunocytochemistry; insulin cell counts were expressed as a proportion of insulin plus glucagon cells. With serum-containing medium, Matrigel stimulated a significant increase in this proportion as compared with collagen gel—3.1% as against 0.2%; the serum-free medium further increased this proportion to 17.3%. Raising the level of essential amino acids approximately fivefold increased the latter figure somewhat (to 18.9%), but it was more than doubled (to 37.4%) by raising the glucose concentration from 10 mM to 20 mM. Raising the levels of amino acids and glucose simultaneously yielded a lesser increase (to 31.8%). Some cultures grown in collagen gel and serum-containing medium for 7 d were transferred to Matrigel and serum-free medium for a further 7 d. Insulin cell development recovered, indicating that progenitor cells had survived and were stimulated to develop by the improved conditions. This study indicates that components of the biomatrix and the medium (in particular, a raised glucose concentration) are important for the survival and differentiation of embryonic insulin cells.  相似文献   

20.
探索恒河猴骨髓间质干细胞(MSC)的体外分离培养方法,为其应用提供实验基础。取恒河猴骨髓细胞悬液,经梯度离心去除大部分血细胞,取含有MSC的中间单核细胞层,在含10%胎牛血清及1ng/mL碱性成纤维细胞生长因子的L-DMEM中培养扩增,并不断换液去除杂细胞,经过18d的原代培养,获得呈致密单层生长的MSC,其形态为较规则的长梭形细胞,排列有方向性,呈现一定的漩涡状、辐射状生长趋势。将原代细胞以1∶2传代,传代培养后期,细胞增殖速度逐渐变缓,细胞形态逐渐出现三角形、多边形及扁平宽大形等不规则形态。结果显示,恒河猴骨髓间质干细胞可在体外进行传代培养,但需进一步优化其培养条件。  相似文献   

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