小麦雌配子体发育过程中酸性磷酸酶活性定位

在小麦(Triticum aestivum L.)雌配子体发育过程中,胚囊周围邻近的珠心细胞退化降解,并出现很高的酸性磷酸酶反应,特别是合点部分最强。电镜细胞化学定位也表明退化珠心细胞质中有强烈的酸性磷酸酶活力,它们存在于多层环状的胞质结构中,而远离胚囊的非退化珠心细胞中无上述结构,酸性磷酸酶活性仅出现于液泡中。认为珠心细胞的退化是一种自溶现象。从功能大孢子至七细胞胚囊期,胚囊内部胞质酸性磷酸酶活性很低,合点与珠孔两端的反应强度无明显区別。后期成熟胚囊阶段,反足细胞中出现强烈酸性磷酸酶活性,中央细胞次之,而助细胞及卵细胞中很弱。     

黄瓜种子萌发过程中Ca~(2 )分布的变化

采用细胞化学方法 ,研究了黄瓜种子中贮藏Ca2 的分布特点及其在萌发过程中的变化动态。干种子的子叶细胞中贮藏有大量的蛋白体、油脂体 ,Ca2 沉淀颗粒大量分布于胞质、胞间隙以及细胞质膜上。大多数蛋白体中有 1至数个圆球形或椭圆体形含Ca2 的球状晶体。相比之下 ,胚芽和胚根细胞中Ca2 较少。种子萌发早期 ,子叶中的贮藏钙及晶体溶解释放出的Ca2 部分转运到生长发育中的胚芽和胚根中。随着萌发的继续 ,胚根和胚芽细胞中的Ca2 不会持续增多 ,反而下降     

黄瓜种子萌发过程中Ca^2＋分布的变化

采用细胞化学方法,研究了黄瓜种子中贮藏Ca^2 的分布特点及其在萌发过程中的变化动态,干种子的子叶细胞中贮藏有大量的蛋白体,油脂体,Ca^2 沉淀颗粒大量分布于胞质,胞间隙以及细胞质膜上,大多数蛋白体中有1至数个圆球形或椭圆体形含Ca^2 的球状晶体,相比之下,胚芽和胚根细胞中Ca^2 较少,种子萌发早期,子叶中的贮藏钙及晶体溶解释放出的Ca^2 部分转运到生长发育中的胚芽和胚根中。随着萌发的继续,胚根和胚芽细胞中的Ca^2 不会持续增多,反而下降。     

黄瓜种子萌发过程中Ca2+分布的变化

采用细胞化学方法,研究了黄瓜种子中贮藏Ca2+的分布特点及其在萌发过程中的变化动态.干种子的子叶细胞中贮藏有大量的蛋白体、油脂体,Ca2+沉淀颗粒大量分布于胞质、胞间隙以及细胞质膜上.大多数蛋白体中有1至数个圆球形或椭圆体形含Ca2+的球状晶体.相比之下,胚芽和胚根细胞中Ca2+较少.种子萌发早期,子叶中的贮藏钙及晶体溶解释放出的Ca2+部分转运到生长发育中的胚芽和胚根中.随着萌发的继续,胚根和胚芽细胞中的Ca2+不会持续增多,反而下降.     

在萌发前后小麦种子糊粉层细胞内酸性磷酸酶的细胞化学研究

采用GMA低温包埋方法和β-甘油磷酸钠为底物,对小麦糊粉细胞在不同萌发时期的酸性磷酸酶活性,进行了细胞化学光学显微镜定位。发现,酸性磷酸酶的活性反应物,大量地存在小麦的干种子糊粉细胞的内壁,胞间,胞间连丝和糊粉粒内。当种子吸水萌发后,存在糊粉细胞内和内壁的酸性磷酸酶,便不断地释放出来,流入胚乳。有关酸性磷酸酶怎样从糊粉细胞流入胚乳的途径,我们提出了一些初步的看法。     

酸性磷酸酶参与大豆子叶磷转运和利用

本文以磷效率不同的两个大豆品种为材料,研究大豆幼苗期子叶酸性磷酸酶活性和同工酶谱对外源磷有效性的响应,及其参与子叶磷高效转运和利用的过程。结果表明：在幼苗生长前期,子叶酸性磷酸酶活性及其同工酶谱组成变化明显,而且不受外源磷有效性的调控;在幼苗生长的前8天,子叶全磷含量随着酸性磷酸酶的活性增加而显著降低,而且磷高效大豆品种比磷低效大豆品种具有较高的酸性磷酸酶活性和植株全磷含量。以上结果说明在大豆幼苗生长前期,由于大粒种子不仅具有较高的磷含量,而且具有较高子叶酸性磷酸酶活性,促进子叶有机磷的水解和转运是磷高效大豆品种适应低磷胁迫的生理机制之一。     

百合花粉母细胞间细胞融合期间腺苷三磷酸酶活性的细胞化学定位及其与染色质胞间转移的关系

用标准的磷酸铅沉淀的细胞化学方法,对百合花粉母细胞间染色质穿壁运动期间及其前后三个时期中的腺苷三磷酸酶(ATP 酶)活性进行了超微结构的定位。结果表明:(1)在穿壁前,ATP 酶活性主要定位于质膜、胞间连丝及细胞间隙;在内质网、高尔基体、质体和某些局部的基质(groundplasm)中,也表现有 ATP 酶活性反应的产物;但在染色质和核仁中,一般都没有这种反应。(2)在穿壁时,染色质从一个细胞穿壁转移到另一个相邻细胞,同时看到染色质和核仁内出现密集的 ATP 酶活性反应产物;在内质网和高尔基体的腔内以及质体的片层上也产生明显的 ATP 酶活性反应;而在质膜、胞间连丝及细胞间隙内 ATP 酶活性明显降低,甚至看不到明显的活性反应。(3)在穿壁后,质膜及细胞间隙中又产生明显的 ATP 酶活性反应产物,但核内染色质上的 ATP 酶活性则显著降低,而核仁内则仍有较高的活性。同前二个时期一样,内质网、高尔基体和质体上的 ATP 酶仍表现明显的活性反应。最后讨论了三个不同发育时期 ATP 酶活性及其分布部位的改变与染色质胞间转移的关系。     

外源激素对大豆种子内源ABA水平的影响及其和同化物积累的关系

用微注射法将ＩＡＡ、ＧＡ３、ＫＴ引入开花后３０ｄ的大豆（ＧｌｙｃｉｎｅｍａｘＬ．）完整植株种子的两片子叶之间,７ｄ后取样,分别测定了种皮和子叶中的ＡＢＡ含量、酸性转化酶和ＡＴＰ酶活性,同时分析了子叶中的糖和蛋白质含量的变化。结果表明：１０－６ｍｏｌ／ＬＩＡＡ和１０－６ｍｏｌ／Ｌ的ＫＴ处理使种皮中的ＡＢＡ水平升高,酸性转化酶活性提高,而ＡＴＰ酶活性降低;相反,对照子叶中的ＡＢＡ水平下降,酸性转化酶活性也下降,而ＡＴＰ酶活性显著提高;１０－６ｍｏｌ／ＬＧＡ３的作用正相反,使种皮和子叶中的ＡＢＡ水平均下降,酸性转化酶活性及子叶中的ＡＴＰ酶活性也相应下降,但种皮中的ＡＴＰ酶活性却上升;子叶中的糖和蛋白质含量的变化没有明确的规律。内源ＡＢＡ含量的变化与转化酶和ＡＴＰ酶活性变化呈现一定的相关关系,表明ＡＢＡ参与了调节大豆种子中的同化物积累。对外源激素对大豆种子内源ＡＢＡ水平的影响及其和同化物积累的关系进行了讨论。     

低温下水稻幼苗叶片细胞膜膜脂过氧化和膜磷脂脱酯化反应

水稻幼苗遭遇冷胁迫（１℃,光照强度１５０μｍｏｌ·ｍ－２·ｓ－１）２ｄ,其叶片丙二醛（ＭＤＡ）含量明显增加,酸性磷酸酯酶活性也增加,同时无机磷含量也增加。３０ｍｍｏｌ／Ｌ的ＣａＣｌ２浸泡种子１ｄ则削弱了冷胁迫的这种作用。Ｈ２Ｏ２和甲基紫精（ＭＶ）均有刺激幼苗叶片和离体根质膜酸性磷酸酯酶活性的作用。     

朱顶红生殖细胞胞质分裂的两种方式(英文)

大多数植物以形成细胞权方式完成胞质分裂过程,也有些植物以类似于动物和单细胞植物在赤道区形成收缩沟的方式而分成两部分。本工作应用电镜对朱顶红体外萌发９～１８小时花粉管中的生殖细胞胞质分裂进行了研究。结果表明：７０％的细胞表现的是第一种方式、３０％却是第二种方式。即：朱顶红生殖细胞胞质分裂同时存在两种方式。前者最初以细胞板亚单位的形式出现于有丝分裂晚后期,它们聚集于成膜体的中央区域并于分裂末期融合成一个大的连续的单位（Ｆｉｇ．１～３）。大量新的微管形成于两组染色体之间（Ｆｉｇ．１）。分裂末期,细胞板形成并具胞质通道（Ｆｉｇ．２）。成膜体微管规则排列并穿过胞质通道向新形成的末期核伸展（Ｆｉｇ．２＆３）。这些微管与构成细胞板的质膜紧密联系（Ｆｉｇ．３）。后者则在有丝分裂后期开始（Ｆｉｇ．４）,当两群染色体彼此分离时,生殖细胞质膜在中央区由两侧向内凹陷形成收缩沟。有时生殖细胞几乎被收缩沟分成两个部分（Ｆｉｇ．６）。发生缢缩的细胞中细胞器与具细胞板的无差异,但微管稀少并且排列紊乱（Ｆｉｇ．４＆５）,染色体的状态使得难以准确区分细胞分裂时期。而且核膜的形成似乎始于有丝分裂后期、出现于染色体边缘（Ｆｉｇ．７）。有时尚有落后     

Ultrastructural Localization of Acid Phosphatase Activity in Soybean Cotyledon Cells

In the cotyledon cells of the developing seeds (35～50 d after flowering) and the early germinating seeds (4 ～ 8 d after sowing) of soybean (Glycine max L. ), acid phosphatase (APase) activity was mainly deposited in the protein bodies (PB) and in endoplasmic reticulum (ER). In addition, in the early developing cotylendon cells, the prominent reaction product of APase activity was seen along the plasma membrane, in the cell wall and within the vesicles in the cytoplasm adjancent to the plasma membrane. And some of the vesicles seemed to be fused with the plasma membrane.     

Late events in B cell activation. Expression of membrane alkaline phosphatase activity

Alkaline phosphatase (APase) has been previously described as a membrane marker correlating with B cell proliferation after stimulation by selected B cell mitogens. We have found, however, that the appearance of B cell membrane APase correlates more closely with differentiation than with proliferation. This conclusion has been drawn from the following observations: 1) APase activity appears well after peak B cell thymidine uptake, 2) mitogens which stimulate only B cell proliferation (Salmonella typhimurium mitogen) fail to induce expression of the enzyme, and 3) when proliferation of mitogen-activated B cells is inhibited, APase activity is not suppressed and may even be augmented. In addition to membrane expression, APase is also spontaneously shed into the surrounding milieu, perhaps as a result of endogenous phospholipase activity. By using a group of well-characterized inhibitors, the APase activity was shown to belong to class I (similar to the bone/liver/kidney class). Because APase always appears in differentiating but not proliferating cells, we would propose that the enzyme appearance is a late marker of B cell activation, associated with cell progression to differentiation and consequent IgM synthesis.     

Transport of acid phosphatase to lysosomes does not involve passage through the cell surface

In foregoing studies, we reported that LGP107, a major lysosomal membrane glycoprotein in the rat liver, distributes in and circulates continuously throughout the endocytic membrane system (endosomes, lysosomes and plasma membrane), in hepatocytes (1,2). In the present study we examined whether acid phosphatase (APase), an enzyme that is transported to lysosomes as a transmembrane protein, passes through the cell surface during intracellular transport, because transport of newly synthesized APase to lysosomes involves the passage of endosomes containing a ligand which is internalized via receptors on the cell surface and is finally dispatched to lysosomes for degradation (3). When localization of APase in rat hepatocytes was investigated by immunoelectron microscopy, APase was found to be localized in lysosomes and endosomes, but not in coated pits on the cell surface, which are positive for LGP107, and from which antibodies for LGP107 are internalized. Further, unlike LGP107, newly synthesized APase was not detected in plasma membranes isolated from livers of rats given [35S]methionine, and when cultured hepatocytes were exposed to 125I-labeled anti APase IgG at 37 degrees C, there was no transfer of the antibody to lysosomes even after 24 h incubation. Therefore, these results indicate that intracellular movement of APase does not involve cell surface passage in rat hepatocytes, and clearly differs from the recent report that human APase is transported to lysosomes via the cell surface in BHK cells transfected with its cDNA (4).     

杜仲次生木质部分化和脱分化过程中酸性磷酸酶的超微细胞化学定位

杜仲（EucommiaulmoidesOliv．）次生木质部分化过程中,在形成层刚衍生的木薄壁细胞中,酸性磷酸酶（APase）主要分布于核膜边缘和高尔基体;在分化程度较高的木薄壁细胞中,APase散布于整个核中,进而,在各种细胞器残体上聚集;在成熟的木薄壁细胞中,APase沿细胞壁内侧分布。在未成熟导管分子中,核、质膜及纹孔上明显存在APase聚集,进而,核解体;在即将分化成熟的导管分子中,APase主要集中于初生壁;在已分化成熟的导管分子中,APase集中于次生壁。脱分化过程中,只在细胞质中可见分散的APase活性,而细胞核和细胞壁上未见此酶的分布;更深层的即将分化成熟和已分化成熟的导管分子,未见有细胞分裂,其上APase的分布与剥皮前相同。通过比较分化和脱分化过程中APase的分布,推测不同的APase同工酶可能分别参与了次生木质部细胞程序性死亡过程中原生质体的解体和次生壁的建成。APase的聚集程度可能是决定细胞能否脱分化的一个重要特征。     

Aquaporins and unloading of phloem-imported water in coats of developing bean seeds

Nutrients are imported into developing legume seeds by mass flow through the phloem, and reach developing embryos following secretion from their symplasmically isolated coats. To sustain homeostasis of seed coat water relations, phloem-delivered nutrients and water must exit seed coats at rates commensurate with those of import through the phloem. In this context, coats of developing French bean seeds were screened for expression of aquaporin genes resulting in cloning PvPIP1;1, PvPIP2;2 and PvPIP2;3. These genes were differentially expressed in all vegetative organs, but exhibited their strongest expression in seed coats. In seed coats, expression was localized to cells of the nutrient-unloading pathway. Transport properties of the PvPIPs were characterized by expression in Xenopus oocytes. Only PvPIP2;3 showed significant water channel activity (Pos = 150-200 microm s(-1)) even when the plasma membrane intrinsic proteins (PIPs) were co-expressed in various combinations. Permeability increases to glycerol, methylamine and urea were not detected in oocytes expressing PvPIPs. Transport active aquaporins in native plasma membranes of seed coats were demonstrated by measuring rates of osmotic shrinkage of membrane vesicles in the presence and absence of mercuric chloride and silver nitrate. The functional significance of aquaporins in nutrient and water transport in developing seeds is discussed.     

一种特殊的长寿细胞:毛竹茎秆纤维细胞

利用显微和细胞化学方法,对毛竹(Phyllostachys edulis)茎秆纤维次生壁形成过程中超微结构变化以及ATP酶、Ca2 -ATPase和酸性磷酸酶的超微细胞化学定位进行了研究.研究发现,次生壁形成早期,细胞核具有双层核膜,染色质凝聚,可见大量的线粒体、粗面内质网和高尔基体等细胞器存在于纤维细胞中;随后,双层核膜消失,细胞器将逐渐解体,多泡体开始出现在纤维细胞的细胞质;随着年龄的增加,纤维细胞壁逐渐增厚,并出现多层结构现象,而运输小泡、细胞膜、胞间连丝和凝聚的染色质将持续存在.在次生壁形成的整个过程中,ATP酶、Ca2 -ATPase和酸性磷酸酶在运输小泡、细胞膜、质膜内陷、胞间连丝和凝聚的染色质中将持续存在.结果表明,毛竹茎秆纤维细胞是一种不同于木本双子叶植物的长寿细胞,纤维原生质体中ATP酶和酸性磷酸酶的持续存在与次生壁的持续增厚密切相关.     

蒜鳞片薄壁细胞衰退过程中酶的细胞化学定位及DNA生化分析

蒜在储藏过程中,鳞茎薄壁细胞衰退,其营养物质供给幼芽萌发生长。采用细胞化学方法,对蒜休眠进程中的鳞茎薄壁细胞进行了ATPase以及APase的细胞化学定位,结果显示在薄壁细胞的质膜、细胞壁和胞间连丝上的酶活性随着蒜自休眠至萌发的不同发育进程而呈现增强的趋势,且在萌芽期酶活性表现最为强烈,表明细胞内物质的降解、转化与输出的加强有助于细胞内含物向新生芽的彻底转移。配合采用琼脂糖凝胶电泳对衰退薄壁细胞的DNA进行了分析,实验结果表现出典型的DNA Ladder,为蒜鳞茎薄壁细胞的衰退属于受基因控制的程序性死亡范畴补充了生化证据。     

P-glycoprotein substrate transport assessed by comparing cellular and vesicular ATPase activity

We compared the P-glycoprotein ATPase activity in inside-out plasma membrane vesicles and living NIH-MDR1-G185 cells with the aim to detect substrate transport. To this purpose we used six substrates which differ significantly in their passive influx through the plasma membrane. In cells, the cytosolic membrane leaflet harboring the substrate binding site of P-glycoprotein has to be approached by passive diffusion through the lipid membrane, whereas in inside-out plasma membrane vesicles, it is accessible directly from the aqueous phase. Compounds exhibiting fast passive influx compared to active efflux by P-glycoprotein induced similar ATPase activity profiles in cells and inside-out plasma membrane vesicles, because their concentrations in the cytosolic leaflets were similar. Compounds exhibiting similar influx as efflux induced in contrast different ATPase activity profiles in cells and inside-out vesicles. Their concentration was significantly lower in the cytosolic leaflet of cells than in the cytosolic leaflet of inside-out membrane vesicles, indicating that P-glycoprotein could cope with passive influx. P-glycoprotein thus transported all compounds at a rate proportional to ATP hydrolysis (i.e. all compounds were substrates). However, it prevented substrate entry into the cytosol only if passive influx of substrates across the lipid bilayer was in a similar range as active efflux.     

Caspase 8 activity in membrane blebs after anti-Fas ligation.

Previous studies of thymocyte apoptosis using a series of cell-permeable fluorogenic peptide substrates showed that Fas cross-linking triggered a caspase cascade in which cleavage of the IETDase (caspase 8-selective) substrate was the earliest caspase activity measured by flow cytometry. This result was expected in light of the abundant evidence for caspase 8 activation as an initiating event in the Fas death pathway. However, when apoptosis was induced by anti-Fas in CTL and the caspase cascade examined by this approach, IETDase activation followed increases in LEHDase, YVHDase, and VEIDase activities (selective for caspases 9, 1, and 6, respectively). When examined by confocal microscopy, anti-Fas-treated CTL showed the early appearance of IETDase-containing plasma membrane vesicles and their release from the CTL surface, followed by activation of other caspase activities in the cell interior. Since these vesicles were not included in the flow cytometry analysis, the early IETDase activity had been underestimated. In contrast to anti-Fas, induction of apoptosis in these CTL by IL-2 withdrawal resulted in early IETDase activity in the cytoplasm, with no plasma membrane vesiculation. Thus, anti-Fas-induced initiation of caspase activity at the plasma membrane may in some cells result in local proteolysis of submembrane proteins, leading to generation of membrane vesicles that are highly enriched in active caspase 8.     

Electron microscope histochemical localization of alkaline phosphatase(s) in Bacillus licheniformis.

Sites of alkaline phosphatase (APase) activity in a facultative thermophilic strain of Bacillus licheniformis MC14 have been localized by electron microscope histochemistry, using a lead capture method. The effects of 3% glutaraldehyde and 3.0 mM lead on APase activity were investigated, and these compounds were found to significantly inhibit enzyme activity, 68 and 18%, respectively. A number of parameters were varied in studies to localize APase activity, including: growth temperature (55 and 37 degrees C); substrate concentration in the histochemical mixture (0.06, 0.15, 0.30, 1.00 mM); fixatives; protoplast preparations and whole cells; phosphate-repressed and -derepressed cells; and age of vegetative cells (mid-log and late log). These variations affected the number but not the location of lead phosphate deposits, which appeared at discrete sites along the inner side of the cytoplasmic membrane. Control cells incubated in histochemical mixtures lacking substrate, lead, or both exhibited no lead phosphate depositis. The histochemical localization at membrane sites correlated well with biochemical localization data, which indicated that greater than 80% of the APase activity was associated with the membrane fraction in logarithmically growing cells.