Actin and myosin during pollen germination

Actin and myosin from pollen tubes of Lilium davidii were studied by using immunoblotting, Dot_Blot and myosin Ca 2+_ATPase analysis. On immunoblotting of the total soluble pollen tube proteins, anti_α_actin antibody labelled a polypeptide approximately 43 ku, which is considered to be the actin of lily. The mRNA encoding actin in ungerminated pollen and germinated pollen were both undetectable in our experiments. A myosin exhibited Ca 2+_ATPase activity, with a native molecular weight of 460 ku has been identified by using immunoblotting. A polypeptide of about 205 ku and a polypeptide of about 20 ku were the heavy chain and a set of light chain of the myosin, which can crossreact with anti_skeletal muscle myosin heavy chain monoclonal antibody and anti_skeletal muscle myosin light chain (20 ku) monoclonal antibody, respectively. The Ca 2+_ATPase activities of myosin in crude extracts of germinated pollen were positively related to the growth rates of pollen tubes.     

Effect of calcium ions on the secondary structures of photosystem II and its relations with photoinhibition

Calcium ions play an important role in the oxygen-evolving process of photosystem II as demonstrated in many experiments. The changes of the secondary structures of PS II induced by the depletion of Ca²⁺ were reported. The results indicated that the removal of Ca²⁺ led to the transition of ahelix to turns and sheet structures. While Ca²⁺ was re-added to the media, only the structures changed to turns could be recovered. The protein conformational changes of PS II during the donor side photoinhibition induced by the depletion of ca²⁺ were also studied. This showed that the protein conformational changes differed between the control and Ca²⁺-depleted samples in a short period of illumination (within 10 min). However, the changes became similar when the illumination time was increased.     

Activities and properties of calcineurin catalytic domain

Calcineurin (CN) is the only protein phosphatase known to be under the control of calcium (Ca²⁺) and calmodulin (CaM). The enzyme consists of two subunits, the catalytic A subunit of 61 ku (CNA) and a regulatory B subunit of 19 ku (CNB). In this study, we used PCR amplication to construct a truncation consisting of only the CNA catalytic domain. The truncation was induced by IPTG and expressed inE. coli. PNPP was used as a substrate to study the phosphatase activity of the CNA catalytic domain. The findings show that its activity is 20 times greater than CNA in the presence of CNB and CaM. The optimum reaction temperature for the CNA catalytic domain protein is 40°C, and the optimum reaction pH value is 8.0. Mn²⁺ is still an effective activator for the CNA catalytic domain, but its activity is not controlled by Ca²⁺. In the presence of 6 mmol/L Mg²⁺, adding either Ca²⁺ or EGTA did not change the activity of the CNA catalytic domain.     

Action mechanisms of a new erythrocyte-derived depressing factor

To investigate the action mechanisms of a new erythrocyte-derived depressing factor (EDDF), the focus is placed on the effect of EDDF on both cytosolic and nuclear free calcium (Ca²⁺) transportation in vascular smooth muscle cell (VSMC), as well as the apoptosis and cell cycle of VSMC of rats. EDDF has been extracted from human erythrocytes. The changes of Ca²⁺ levels in cytoplasm ([Ca²⁺]_i) and nucleus ([Ca²⁺]_n) have been observed using a laser scanning confocal microscope together with fluo-3/AM as a calcium indicator. Flow cytometric technique was used to study the effect of EDDF on cell cycle and apoptosis of VSMC. [Ca²⁺], and [Ca²⁺]_n were significantly decreased through several different pathways: ( i ) it reduced the Ca²⁺ influx by blocking L-type voltage-dependent calcium channel (L-VDC) and R-type voltage-dependent calcium channel (R-VDC); (ii) it inhibited the Ca²⁺ release from inositol 1, 4, 5-trisphosphate (IP₃) sensitive calcium store; and (iii) activated Ca²⁺-ATPase of sarcoplasmic reticulum (SR) and promoted the transportation of Ca²⁺ from cytoplasm to SR. However, EDDF seemed to have little inhibitory effect on the Ca²⁺ release from ryonodine sensitive calcium pool. It was also found that EDDF (10⁻⁴ g/mL) significantly decreased the proportion of S phase of human umbilical vein (HUV) and inhibited the proliferation of VSMC induced by angiotensin II (Angll, 10⁻⁵ mol/L). The apopotosis did not occur when VSMC was cultured under normal condition. While VSMC apoptosis was induced by Angll (10⁻⁵ mol/L) and EDDF (10⁻⁴ g/mL) seemed to have little effect on it. The inhibitory effect of EDDF on the elevation of [Ca²⁺]_i and [Ca²⁺]_n of VSMC might play an essential role in its action mechanisms and the ways it affects the Ca²⁺ handling of VSMC demonstrate that EDDF was different from other endogenous blood pressure regulators and some known antihypertensive drugs. EDDF could inhibit the proliferation of VSMC, which indicated that it might be beneficial to the prevention and treatment of hypertension and arteriosclerosis.     

Identification of a DNase activated inXenopus egg extracts undergoing apoptosis

A cell-free apoptosis system was established by adding dATP and cytochrome c toXenopus laevis egg extracts S-150. Accompanied by an incubation process, an apoptosis-specific DNase was activated in egg extracts which depended on Mg²⁺ and inhibited by Zn²⁺. Two nucleases existing in egg extracts were revealed by in-gel nuclease assay. Further experiments showed that 27 ku nuclease which was different from other Ca²⁺ /Mg²⁺ -dependent nucleases was a possible candidate involved in apoptosis.     

Role of Ubisch bodies secreted by tapetum in Ca2+ transprot

The distribution of Ca²⁺ in the anthers of wheat was observed using cytochemical method of potassium antimonite. At the later tetrad stage, Ubisch bodies carrying Ca²⁺ were observed on the inner surface of tapetum, in anther locule and on pollen surface. The Ubisch bodies contacted with pollen, and Ca²⁺ began to accumulate on pollen surface. At the uninucleate pollen stage, abundant Ubisch bodies were distributed in anther locule, and the amount of Ca²⁺ on pollen surface increased. At the mature pollen stage a large amount of Ca²⁺ ions were localized on the inner surface of tapetum, the surface of pollen and Ubisch bodies. In the pollen wall, Ca²⁺ precipitates arranged in radial lines. These results demonstrated that Ubisch bodies were involved in Ca²⁺ transport from anther wall to pollen surface at some developmental stages of anther.     

The binding of the anticoagulation factor Ⅰ from the venom of Agkistrodon acutus to activated factor Ⅹ

Anticoagulation factor Ⅰ (ACF Ⅰ) from the venom of Agkistrodon acutus prolonged plasma prothrombin time (PPT) with dose-dependent manner and exhibited marked anticoagulant activity only at the concentration higher than its critical concentration (12 nmol/L). It was discovered that ACFⅠ formed a 1:1 complex with activated coagulation factor (FⅩa) in the presence of Ca2+ ions by the method of polyacrylamide gel electrophoresis. Both native ACFⅠ and decalcified ACFⅠ failed to form complexes with FⅩa in the absence of Ca2+. Sr2+ ions were able to replace Ca2+ ions in the binding of ACFⅠ to FⅩa, but both Ba2+ ions and Tb3+ ions were ineffective. ACFⅠ was a new member of the Ⅸ/Ⅹ-bp family in the C-type lectin superfamily, and had a amino acid composition similar to the other members of this family. It was composed of 251 amino acid residues with a molecular weight of 29 603.6 u on non-reducing condition, determined by MALDI-TOF-MS, and a molecular weight of 14.7 ku on reducing condition, determined by the sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE).     

Cardiac protective role of a novel erythrocyte-derived depressing factor on rats and its Ca^2＋ mechanism

The cardiac protective role of a novel erythro-cyte-derived depressing factor (EDDF) on spontaneous hy-pertensive rats (SHR), calcium overload (CaO) rats and Wistar rats and its mechanism was evaluated. Mean artery pressure (MAP), heart rate (HR) and LVdp/dtmax were measured by physiological recorder. The effect of EDDF on the Ca2+-ATPase activity in myocardial sarcoplasmic reticu-lum (SR) of CaO rats was determined by inorganic phos-phate assay. Calcium transport in myocytes was measured by 45Ca2+ radioactive isotope measurement. The phosphoryla-tion levels of extracellular signal-regulated protein kinases (ERK1/2) in myocardial tissue of SHR and CaO rats were measured by Western blot method. And the ultrastructures of cardiac muscle cells were observed with the transmission electron microscope. The results indicated that EDDF could significantly decrease MAP, HR and LVdp/dtmax in a dose dependent manner (P < 0.05). It seems that the mechanism might relate with activating the Ca2+-APTase, enhancing the uptake and release of Ca2+ from SR (P < 0.05), decreasing the phosphorylation levels of ERK1/2 of myocytes (P < 0.01) and lightening the ultrastructural lesion of cardiac muscle cells. In CaO rats, the Ca2+-ATPase activity decreased clearly com-pared to control (64.99 7.16 vs 94.48 7.68 nmol·min-1 ·mg-1 protein, P < 0.01), while EDDF (100 mg/mL) could significantly increase the activity (87.93 ?9.54 vs 64.99 ?7.16, P < 0.05, n = 7). Both uptake and release rate of Ca2+ (祄ol 45Ca2+/g protein/min) from myocardial SR of CaO rats re-markably decreased compared to control (32.40 ?2.70 and 15.46 ?1.49 vs 61.09 ?10.89 and 25.47 ?4.29, P < 0.05); EDDF (100 mg/mL) could significantly stimulate their activi-ties (50.48 6.76 and 21.76 2.75 vs 32.40 2.70 and 15.46 1.49, P < 0.05). EDDF could evidently down-regulate the phosphorylation of ERK1/2 in myocardial tissue from SHR and CaO rats (P < 0.01), lighten the ultrastructural lesion of cardiac muscle cells of SHR as well. It is concluded that EDDF seems to play protective roles on both structure and function of heart, which closely related with amelioration of Ca2+ transport and inhibition of Ca2+-MAP kinase pathway.     

热敏灸对运动大鼠运动能力和心肌、骨骼肌细胞线粒体过氧化损伤的影响

目的研究热敏灸对运动大鼠运动能力和心肌、骨骼肌细胞线粒体过氧化损伤的影响。方法将40只大鼠随机分为正常对照组、单纯运动组、运动+普通悬灸组和运动+热敏灸组,采用14 d递增大强度跑台运动训练和生物化学的方法,观察热敏灸对运动大鼠运动能力和心肌、骨骼肌细胞线粒体过氧化损伤的影响。结果运动+热敏灸组大鼠疲劳相关症状显著改善,跑台力竭时间显著高于运动+普通悬灸组和单纯运动组。运动+热敏灸组大鼠心肌、骨骼肌细胞线粒体SOD酶活性高于单纯运动组、运动+普通悬灸组,心肌细胞线粒体SOD酶活性低于正常对照组,但骨骼肌细胞线粒体SOD酶活性与正常对照组比较,差异无显著性;MDA含量低于单纯运动组和运动+普通悬灸组,但高于正常对照组。结论热敏灸足三里穴具有明显的抗运动性疲劳作用,机理与热敏灸降低过度运动大鼠心肌和骨骼肌细胞线粒体过氧化损伤有关。     

Phosphatidylglycerol effect on oxygen-evolving activity in Ca2+-depleted photosystem II

The effect of anionic phosphatidylglycerol (PG) on oxygen evolution in a photosystem II (PS II ) particle depleted of Ca²⁺ (designated d_CaPSII ) has been investigated. The major finding is the observation of a new role of PG in the PSII function. That is, PG restores nearly the lost oxygen evolution in d_caPS II particle owing to Ca²⁺ depletion to the levels in intact PS II. Furthermore, there is a stimulation of oxygen-evolving activity in the d_CaPSII complexed with PG in the presence of exogenous CaCl₂, which PG enhances increasingly oxygen evolution with increasing CaCl₂ concentration. It is suggested that PG-induced oxygen evolution recovery of d_Ca PS II particle results from resumption of normal structure in protein by PG effect, whereas the enhancement of oxygen evolution in complex subject to CaCl₂ is ascribed to the optimization of such a structure due to coordination complex formation of Ca²⁺ ions with PG.     

Mg2+-induced LHC II aggregation in thylakoid membrane

Mg²⁺-induced changes in 77K fluorescence spectra of wheat thylakoid membranes were analyzed by a Gaussian deconvolution program. All spectra were fitted well with 7 Gaussian sub-bands. The sub-band areas for the LHC H macroaggregate (F₆₉₉) and PS II (F₆₈₅ and F₆₉₅) were increased and those for the LHC II trimer (F₆₈₁) and PS I (F₇₂₉ and F₇₄₀) were decreased by Mg²⁺. Moreover, it was found that the sub-band area ratio for F₆₉₉ over F₆₈₁ was dramatically enhanced by Mg²⁺ by 1.72 times. It was concluded that the LHC II trimer in thylakoid membranes could be aggregated and transformed into its macroaggregate by Mg²⁺ on a large scale. The possible implication of the Mg²⁺-induced LHC II aggregation was also discussed.     

The new sideway of CNTF signal transduction pathway

The action of ciliary neurotrophic factor (CNTF) on intercellular free Ca²⁺ concentrations [Ca²⁺]_i induced by glutamate (Glu) in primary cultured hippocampal neurons were detected with Fura2/AM, a Ca²⁺-sensitive fluorophore, and the morphological influence of G-protein on it was objected. Glu could induce rapid increase of [Ca²⁺]_i in hippocampal neurons. CNTF had no significant action on [Ca²⁺]_i in resting hippocampal neurons. However, after incubation of CNTF for 5 min, the increase of [Ca²⁺]_i in hippocampal neurons rapidly induced by Glu was inhibited. Pretussis toxin (PTX)-sensitive G protein could block the action. These results indicate that a new non-genomic rapid sideway might exist in the upper stream of CNTF signal transduction pathway, which was related to Ca²⁺ signal transduction. Keywords:     

Effect of Ca on CO2 corrosion properties of X65 pipeline steel

The effect of Ca²⁺ on CO₂ corrosion to X65 pipeline steel was investigated in the simulated stratum water of an oil field containing different concentrations of Ca²⁺. It is found that Ca²⁺ can enhance the corrosion rate, especially in the Ca²⁺ concentration from 256 to 512 mg/L, which can be attributed to the growing grain size and loosing structure of corrosion scales with increasing Ca²⁺ concentration. X-ray diffraction (XRD) and X-ray photoelectron spectroscopy (XPS) investigations reveal that a complex carbonate (Fe, Ca)CO₃ forms at high Ca²⁺ concentration due to the gradual replacement of Fe²⁺ in FeCO₃ by Ca²⁺.     

Myosin isoenzyme redistribution in chronic heart overload.

Since the first observation by Spann et al., it has become clear that in cardiac hypertrophy induced by a mechanical overloading, the velocity of shortening of the cardiac muscle (Vmax) is reduced (see ref. 2 for review). Most authors agree that this mechanical alteration is accompanied by a decrease in the Ca2+-dependent ATPase activity of myosin (see ref. 3 for review). The molecular basis of such changes was unknown because the structural modifications of the myosin molecule were ill-defined. Nevertheless, it has recently been shown that, like skeletal muscle myosin, cardiac myosin is composed of several polymorphic forms, comparable to isoenzymes. In the skeletal muscle, new functional requirements can induce changes in both contractile activity and type of myosin isoenzyme synthesised. We now report that an increase in cardiac work produced by mechanical overloading in rats induces the preferential synthesis of a cardiac myosin isoenzyme characterised by specific immunological and electrophoretic properties and exhibiting a lower ATPase activity. This adaptive change could account for the reduced shortening speed of this hypertrophied cardiac muscle.     

Effects of La3+ and Gd3+ on Ca2+ influx in rat hepatoma H-35 cells

Effects of La³⁺ and Gd³⁺ on Ca²⁺ influx were investigated in rat hepatoma H-35 cells by measuring the initial rate of⁴⁵Ca²⁺ uptake. It was found that the maximum initial rate of Ca²⁺ uptake was increased six-to ten-fold at low concentrations of La³⁺ and Gd³⁺. Kinetic analyses by measuring the initial rate of Ca²⁺ influx at different external Ca²⁺ concentrations indicated the existence of two intracellular exchangeable components in the basal Ca²⁺ system, with low and high affinities for Ca²⁺, and only one class of Ca²⁺ binding sites was observed in the La³⁺-or Gd³⁺-treated cells. For high affinity, La³⁺ and Gd³⁺ increased both kinetic parametersK _m andV _max of basai Ca²⁺ influx. La³⁺ and Gd³⁺ compete directly with Ca²⁺ for Ca²⁺ binding site for low affinity. The kinetics is competitive.     

Ca2+ signals induced from calcium stores in pancreatic islet β cells

In single rat pancreatic β cells, using fura-2 microfluorometry to measure [Ca²⁺]i response upon different stimuli, the ways of calcium regulation have been studied. When the extracellular calcium concentration was 2.5 mmol/L, either 60 mmol/L KCl, 20 mmol/L D-glucose or 0.1 mmol/L tolbutamide induced increase in [Ca²⁺]i. Such increase in [Ca²⁺]i was absent when the same stimuli were applied under zero extracellular calcium. These results indicate that the increase of [Ca²⁺]i is induced by the activation of voltage-dependent calcium channels in β cells. The manifold forms of [Ca²⁺]i change induced by glucose imply that the effects of glucose are complex. 5 mmol/L caffeine or 5 mmol/L MCh increase the [Ca²⁺]i, which is independent of the external calcium, suggesting that [Ca²⁺]i can be regulated by Ca²⁺ release from not only the IP₃-sensitive but also the ryanodine sensitive calcium stores in β cells. The latency of Ca responses for IP₃ pathway (5 s) is faster than that for ryanodine pathway (30 s). It is concluded that there are multiple calcium stores in rat pancreatic β cells.     

Heat and hyposmotic stimulation increase in [Ca^2＋]i by Ca^2＋ influx in rat synoviocytes

Rheumatoid arthritis （RA）, which is marked by inflammatory synovitis, is a common, chronic autoimmune-disease, whose pathogenesis is complex and still unclear. In order to explore the effects of heat and hyposmotic stimuli on synoviocytes in rheumatoid arthritis, the changes of [Ca^2＋]i induced by heat, hyposmotic and 4α-PDD stimuli were observed in synoviocytes. [Ca^2＋]i elevation induced by heat 28℃, hyposmotic and 4α-PDD stimuli is found to be positively relative to increasing temperature, decreasing osmolality and rising concentration of 4α-PDD. Results show that there is reciprocity among these stimuli and desensitization, and that [Ca^2＋]i elevation depends on Ca^2＋ influx, but not necessarily links to Ca^2＋ release from intracellular stores and voltage-dependent Ca^2＋ channel in synoviocytes. The above characteristics of Ca^2＋ influx are similar to those of TRPV4. A probable mechanism has been suggested that heat and hyposmotic stimulation might increase the level of [Ca^2＋]i by activating the TRPV4-like channel and Ca^2＋ influx in the synoviocytes.     

Mitochondrial response and calcium ion change in apoptotic insect cells induced by SfaMNPV

Mitochondrial responses and changes of calcium ions in apoptotic insect SL-1 cells induced by Syngrapha falcifera multiple nuclear polyhedrosis virus (SfaMNPV) are reported in this paper. By using Rhodamine 123 as a fluorescent labeling probe, flow cytometry analysis and confocal laser scanning microscope observation we observed that the mitochondrial transmembrane potential (△ψm) began to decrease in SL-1 cells at 4 h post infection and △ψm reduced continuously with the extension of virus infection. Western blotting indicated that the Bcl-2 level in the mitochondria gradually declined and was down- regulated. Cells undergoing apoptosis were found to have an elevation of cytochrome c in the cytosol and a corresponding decrease in the mitochondria, which indicated that cytochrome c was released from mitochondria into cytosol. These results suggest that mitochondrion-mediated apoptotic signal transduction pathway exists in apoptotic insect cell induced by SfaMNPV. Cytosolic free calcium ([Ca^2 ]i) concentration rapidly increased after SfaMNPV infection and the elevated calcium was tested to come partly from extracelllular calcium ion influx. Flow cytometry analysis indicated that the apoptosis in SL-1 cells was not influenced by established cytosolic calcium clamped conditions and the EGTA inhibiting calcium influx. Therefore, neither the elevation of cytosolic calcium ion nor extracellular calcium entry was the inducing factor of apoptosis, which hinted that the depletion of ER Ca^2 store contributed to SL-1 cell apoptosis induced by SfaMNPV.     

Relationship between LTP and the nuclear protein induced by calcineurin

Results demonstrate that calcineurin plays a role in long term potentiatibn (LTP) in the hippocampus. A 45 ku enzyme was administered, which exhibits Ca²⁺ /calmodulin independent activity to rats, and the protein components of nuclear extracts from the cell-free system of rat hippocampus were tested. It is found that the level of a component significantly increased in nuclear extracts following the activation of calcineurin. The concentration of the component in the nucleus is also markedly increased following hippocampal LTP elicited by ginsenosides. These results suggest that the activation of calcineurin induces a preexisting protein component to translocate to the nucleus in the hippocampus. The nuclear translocation of the component may be required for LTP in the hippocampus.     

切变速度和Ca~(2+)对再生丝素蛋白溶液构象转变的影响

采用偏光显微镜和拉曼光谱研究了切变速度和Ca2+对再生丝素蛋白水溶液构象转变的影响.结果表明:切变速度和Ca2+是影响再生丝素蛋白溶液性质的两个主要因素,对于同一再生溶液,切变速度增大,溶液中丝素蛋白分子沿切变方向的有序排列也随之增加,丝素溶液更容易从无规线团或α-螺旋向β-折叠转变,并且转变的程度随着剪切速度的增加而加强;透析溶液中Ca2+含量增加,则样品出现偏光现象的临界切变速度有所降低.拉曼光谱显示丝素蛋白分子构象由SilkⅠ向SilkⅡ转变.