不同品种花生种子蛋白质的电泳分析

对中国花生（ＡｒａｃｈｉｓｈｙｐｏｇａｅａＬ．）５种不同类型的４６个栽培品种的种子蛋白质进行电泳分析。ＳＤＳＰＡＧＥ和ＩＥＦＳＤＳＰＡＧＥ（双向电泳）的结果显示,不同品种的花生种子蛋白多肽组成存在４种类型。与初步纯化的花生球蛋白及伴花生球蛋白的ＳＤＳＰＡＧＥ结果比较,花生种子蛋白组成的主要差异在于花生球蛋白亚基组成的不同,其中类型Ⅰ花生球蛋白主要含有４１ｋＤ、３８５ｋＤ和２个１８ｋＤ亚基,类型Ⅱ主要含４１ｋＤ、３８５ｋＤ、３７５ｋＤ和３个１８ｋＤ亚基,类型Ⅲ主要含４１ｋＤ、３８．５ｋＤ、３６．５ｋＤ和３个１８ｋＤ亚基,类型Ⅳ主要含４１ｋＤ、３８．５ｋＤ、３７５ｋＤ、３６．５ｋＤ和３个１８ｋＤ亚基。不同品种的伴花生球蛋白多肽组成基本一致。对不同类型８个品种种子蛋白的氨基酸组成进行测定,发现类型Ⅰ的含硫氨基酸含量较高。     

红苋R104种子谷蛋白的电泳分析

通过单向水平变性聚丙烯酰胺凝胶等电聚焦（ＩＥＦ）、十二烷基硫酸钠聚丙烯酰胺凝胶电泳（ＳＤＳ—ＰＡＧＥ）和双向电泳（ＩＥＦ×ＳＤＳ—ＰＡＧＥ）分析了红苋Ｒ１０４种子谷蛋白的亚基组成,亚基分子量和等电点分布。谷蛋白的双向电泳图谱可分辨出１００多个亚基成分．其主要亚基为：５４ｋＤ（ｐＩ７．１５）;３３ｋＤ（ｐＩ５．８２）;３１ｋＤ（ｐＩ６．９２;ｐＩ６．７０;ｐＩ６．６５）;２２ｋＤ（ｐＩ８．３４）;２０ｋＤ（ｐＩ６．９２;ｐＩ６５６）;１８ｋＤ（ｐＩ６．９２;ｐＩ７３５;ｐＩ７．７２;ｐＩ８．０５）。另外,还对ＩＥＦ方法进行了讨论。     

人肾液泡型H~＋_－ATPase 58kD亚基基因的表达

在大肠杆菌中表达了人肾液泡型Ｈ￣＋－ＡＴＰａｓｅ５８ｋＤ亚基的基因,利用聚合酶链式反应（ＰＣＲ）得到了５８ｋＤ亚基的编码片段．直接将ＰＣＲ产物连接到ＰＥＴ载体上表达．ＳＤＳ聚丙烯酰胺凝胶电泳和蛋白质印迹分析表明５８ｋＤ亚基的基因得到高效表达．表达产物可达细菌细胞质蛋白的５０％．     

圆弧青霉碱性脂肪酶的分离纯化和特性

圆弧青霉突变株ＰＧ３７ 发酵液经离心、硫酸铵盐析、疏水层析、阴离子交换层析和凝胶过滤分离纯化得到了比活性为每毫克蛋白质５ ２００ ｕ 的碱性脂肪酶, 纯化倍数１６ ．５ , 得率３３．２％ , 在聚丙烯酰胺凝胶电泳（ＰＡＧＥ）和ＳＤＳ聚丙烯酰胺凝胶电泳（ＳＤＳＰＡＧＥ）上均呈现单一蛋白质条带。ＳＤＳＰＡＧＥ 和凝胶过滤分别测得酶的分子量为２７．５ ｋＤ和２９ ｋＤ, 表明该酶以单体形式存在。Ｎ末端１０ 个氨基酸的序列测定结果为ＡＴＡＤＡＡＡＦＰＤ, 与已知的碱性脂肪酶的Ｎ 末端序列没有同源性。酶学特性研究结果表明, 该酶的最适作用温度为２５ ℃, 在３０ ℃以下稳定,４０ ℃处理２０ ｍｉｎ 仅残留３０ ％ 酶活性;ｐＨ 稳定范围在６．５～１０．５ , 最适ｐＨ 为１０ ．０ 。低浓度的碱性蛋白酶对ＰＧ３７ 碱性脂肪酶活性的影响较小, 可同时添加在洗涤剂中。     

钙／钙调素依赖性蛋白激酶对17．7kD和6kD胰腺蛋白的磷酸化

本文报导了胰腺提取物中两种可被钙／钙调素依赖性蛋白激酶磷酸化的热稳定蛋白。ＳＤＳ－ＰＡＧＥ测定其表观分子量分别为１７．７ｋＤ和６ｋＤ。经钙／钙调素依赖性蛋白激酶磷酸化后,其最大磷酸参入量为８．８μｍｏｌ／ｇ蛋白。同时磷酸化作用导致１７．７ｋＤ蛋白在ＳＤＳ－ＰＡＧＥ中迁移率发生变化。本文还进一步分析了各种阳离子对磷酸化的影响,并对此两种蛋白可能具有的生理功能进行了初步探讨。     

带3蛋白转运吡啶二羧酸根离子的动力学研究

利用ＤＰＡ使Ｔｂ３＋的荧先强度显著增强的原理进行带３蛋白活性的测定,方法简便、灵敏、重复性好,而且能够进行连续荧光扫描测量．应用连续荧光扫描法测定了带３蛋白介导的ＤＰＡ与Ｃｌ－交换的动力学特征参数．结果表明,带３蛋白介导的ＤＰＡ与Ｃｌ－的交换对ＤＩＤＳ非常敏感,受ＤＩＤＳ的强烈抑制,抑制程度大于９０％;ＤＰＡ由内向外转运的米氏常Ｋｍ＝２８．１—３１．２ｍｍｏｌ／Ｌ;带３蛋白的天然底物Ｃｌ－从内侧竞争性抑制ＤＰＡ向外转运,抑制常数ｋｉ＝６０．４±６．９ｍｍｏｌ／Ｌ;膜内侧ＤＰＡ与外侧Ｃｌ－交换的活化能,在４—２５℃范围内为５．８±０．５ｋＣａｌ／ｍｏｌ２５—３７℃范围内为１９．８±１．５ｋＣａｌ／ｍｏｌ;膜内侧ＤＰＡ与外侧Ｃｌ－交换受转运介质ｐＨ（膜内外对称改变）的显著影响,ｐＨ＜７．４时,交换速度显著升高．本实验证明ＤＰＡ确是经带３蛋白而转运的,但转运机制可能与无机离子转运有所不同。     

血管紧张素II和阿片肽对Fos蛋白表达的影响

利用抗体免疫沉淀技术研究了血管紧张素ＩＩ,δ受体激动剂和ｋ受体激动剂对大鼠脑组织ｃ－ｆｏｓ原癌基因表达的影响,结果表明,０．１μｍｏｌ／Ｌ ＡⅡ可显著刺激脑组织中Ｆｏｓ蛋白的表达,０．１μｍｏｌ／ＬＤＰＤＰＥ和０．１μｍｏｌ／Ｌ ＮＤＡＰ对Ｆｏｓ蛋白的表达亦有一定的诱导作用。ＡＩＩ与ＤＰＤＰＥ或ＮＤＡＰ共同处理组织,Ｆｏｓ蛋白表达水平低于ＡＩＩ单独诱导的水平,结果表明阿片肽可抑制ＡＩＩ对Ｆｏｓ蛋白     

大豆下胚轴可溶性蛋白中钙激活的蛋白激酶

大豆（Ｇｌｙｃｉｎｅ ｍ ａｘ Ｌ．） 下胚轴可溶性蛋白提取液进行自磷酸化，以ＳＤＳ－ＰＡＧＥ电泳分析其标记产物时发现，当有较高浓度的Ｃａ２＋ 存在于反应液中时，有一条１８ ｋＤ蛋白带被高强度标记，同时也可观察到另一条标记强度不高的６７ ｋＤ蛋白带． 当反应时间延长到１５ 或３０ｍ ｉｎ 时，它们的标记强度都逐渐减弱，最终从放射自显影底片上消失；在反应液中加入钙螯合剂ＥＧＴＡ 时，则只有６７ ｋＤ 被高强度标记；在磷酸化反应过程中加入非标记ＡＴＰ，蛋白中的３２Ｐ逐渐被非标记磷取代，表明反应体系处于磷酸化－脱磷酸化的平衡过程中，并有结果显示这一过程是钙依赖性的． 组蛋白Ｈ１ 可以使反应进程加快，表明提取液中的蛋白激酶可以利用它作为底物． 综合结果表明，１８ ｋＤ和６７ ｋＤ蛋白可能是具有自磷酸化能力且对Ｃａ２＋ 敏感的蛋白激酶，它们对Ｃａ２＋ 的不同反应，使得钙信号的传递更具可控性     

红苋P104种子谷蛋白的电泳分析

通过单向不平变性聚丙烯酰胺凝胶等电聚焦（ＩＥＦ）、十二烷基硫酸钠聚丙烯酰胺凝胶电泳（ＳＤＳ－ＰＡＧＥ）和双向电泳（ＩＥＦ×ＳＤＳ－ＰＡＧＥ）分析了红苋Ｒ１０４种子谷蛋白的亚基组成,亚其分子量和等电点分布。谷蛋白的双向电泳图谱可分辨出１００多个亚基成分,其主要亚基为：５４ｋＤ（ｐＩ７．１５）;３３ｋＤ（ｐＩ５．８２）;３１ｋＤ（ｐＩ６．９２;ｐＩ６．７０;ｐＩ６．６５）;２２ｋＤ（ｐＩ８．３４）;２     

优质蛋白玉米胚乳贮存蛋白积累的电泳分析

玉米胚乳的２２ ｋＤ和２０ ｋＤ醇溶蛋白在授粉后１５ 天开始积累,编码２２ ｋＤ 和２０ ｋＤ醇溶蛋白的结构基因在胚乳发育过程中同时表达。优质蛋白玉米和ｏ２ 玉米的胚乳中,２２ ｋＤ和２０ ｋＤ醇溶蛋白的合成受到抑制,即ｏ２ 基因对２２ ｋＤ和２０ ｋＤ醇溶蛋白的合成有负的调节作用。Ｍｏ１７／ｏ２ 和Ｍｏ１７ 胚乳醇溶蛋白的双向电泳结果表明,Ｍｏ１７／ｏ２ 的２７ ｋＤ、２２ ｋＤ、２０ ＫＤ和１５ ｋＤ醇溶蛋白的合成均受到强烈的抑制。遗系０４１／ｏ２ 和遗系０４０／ｏ２ 胚乳醇溶蛋白的双向电泳结果表明,二者只在高分子量的蛋白质斑点区域有一些细微的差别。可溶性蛋白的ＳＤＳ－ＰＡＧＥ分析表明,Ｍｏ１７／ｏ２ 胚乳的可溶性蛋白比其同型系Ｍｏ１７ 少３８．７ ｋＤ 和２６．７ ｋＤ两条谱带,多２７．２ ｋＤ和２６．１ ｋＤ两条谱带。二者出现的可溶性蛋白的差异是ｏ２ 基因调控的结果。遗系０４１／ｏ２ 胚乳的可溶性蛋白比其同型系０４０／ｏ２ 多１８．６ ｋＤ和１７．６ ｋＤ两条谱带,少４０．２ ｋＤ 一条谱带,这与ｏ２ 基因修饰因子的作用密切关联     

二氧化碳浓度升高对太湖沉水植物马来眼子菜生长的影响

通过室外培养试验,研究不同CO₂浓度条件下沉水植物马来眼子菜的生长及生理变化.结果表明：CO₂浓度升高(1000 μmol·mol^-1)条件下,马来眼子菜单株的平均生物量增加了44.3%(P<0.01),茎生物量比重下降了5.5%(P<0.05);根和叶中氮含量分别下降了18.1%和6.4%(P<0.05),而茎中氮含量变化不明显(P>0.05);根、茎、叶中磷含量分别增加了22.2%(P<0.05)、26.6%(P>0.05)和38.8%(P<0.05);可溶性糖含量增加了27.3%、18.3%和37.5%(P<0.05);根、茎和叶中全碳含量增加了4.6%、5.3%和2.0%;CO₂浓度升高使水体中氮、磷含量分别下降了7.9%和5.1%(P<0.05),但对底泥中氮、磷的含量影响不明显.CO₂浓度升高将对沉水植物生长及其生境有一定影响.     

模拟酸雨对不同土壤有机碳和作物秸秆分解的影响

为研究酸雨对不同pH值水稻土中有机碳分解的影响,选择酸性（pH 5.48）、碱性（pH 8.18）和中性（pH 6.70）水稻土（分别设置施用秸秆0、15 g·kg^-1土处理）在20 ℃条件下进行40 d的培养试验,各土壤组分别用pH值为6.0、4.5、3.0的模拟雨水将土壤含水量调为400 g·kg^-1(以风干土计).结果表明：秸秆、酸雨和土壤共同对土壤系统CO₂释放产生影响,秸秆的添加可显著提高土壤CO₂释放速率.培养期间,酸雨未显著影响土壤有机碳分解,但对土壤中作物秸秆的分解影响显著. pH 3.0酸雨处理下酸性和碱性土壤中秸秆40 d总分解量比pH 6.0处理高8%;酸雨抑制了中性水稻土中秸秆的分解,pH 3.0酸雨处理下秸秆40 d总分解量比pH 6.0处理低15%.pH 3.0酸雨处理下,酸性水稻土有机碳分解速率分别比中性和碱性水稻土高43%和50%（P<0.05）,秸秆在中性水稻土中分解量分别比其在酸性和碱性水稻土中低17%和16%（P<0.05）.     

Purification and characterization of placental protein 5

This report describes the purification of placental protein 5, PP5, from the human placenta by two affinity chromatography steps, the first with Heparin-Sepharose and the second with Sepharose-linked monoclonal anti-PP5 antibody. The final purification is achieved by reversed-phase high performance liquid chromatography. In SDS-polyacrylamide gel electrophoresis under reducing or nonreducing conditions, PP5 purified in this study migrates as one major band at 36 kD. The previously purified PP5 is more heterogeneous: under nonreducing conditions it migrates at 30 kD and, after reduction, it gives three bands at 16.8 kD, 18.3 kD, and 19.0 kD. In Western blot analysis, both purified proteins react with polyclonal and monoclonal anti-PP5 antibodies. Three N-terminal amino acid sequences are obtained for the previously purified PP5, whereas the N-terminal of PP5 purified in this study is blocked. These results suggest that PP5 previously purified in the absence of protease inhibitors, does not represent the native form of PP5. Computer comparison of the obtained amino acid sequences revealed no significant homology to known protein sequences.     

A novel 17 kD heparin-binding growth factor (HBGF-8) in bovine uterus: purification and N-terminal amino acid sequence

We have purified to near homogeneity a novel 17 kD growth factor from bovine uterus which we designated heparin-binding growth factor-8 (HBGF-8). The growth factor binds tightly to cation exchange resins and to Heparin-Sepharose and is stable to acetone precipitation and labile in acid. Based upon total activity in acetone extracts of bovine uterus stimulating 3H-thymidine incorporation into DNA of serum-starved NIH 313 cells, a 6940 fold purification was achieved with an overall yield of HBGF-8 activity of 0.4%, using extraction of acetone powders and chromatographic separations at neutral pH. Approximately 18 micrograms protein was obtained from 1.2 kg wet weight of tissue. HBGF-8 was clearly separated from 17.5 kD bovine uterus basic fibroblast growth factor (bFGF) by purification and its N-terminal amino acid sequence analyzed. A polypeptide with a unique 25 N-terminal amino acid sequence was found. HBGF-8 was as active as acidic fibroblast growth factor (aFGF) and slightly less active than bFGF in the mouse NIH 3T3 fibroblast mitogenic assay system with an intrinsic specific activity of 5000 dpm/ng under standard assay conditions.     

Prokaryotic Expression and Bioinformatics Analysis of Cytosolic Malate Dehydrogenase from Camellia sinensis(Theaceae)

The complete gene of cytosolic malate dehydrogenase (cMDH) from Camellia sinensis, called Cs cMDH, was obtained by RT PCR and rapid amplification of cDNA ends (GenBank accession number GQ845406). This gene was 1 235 bp in length, encoding a protein of 332 amino acids with the putative molecular weight of 355 kD. The Ecoli Rosetta (DE3) harboring pGEX MDH was induced by 05 mmol·L 1 IPTG at 32℃ for 3 hours, and a 615 kD glutathione Stransferase (GST) fused MDH was obtained in soluble form. The results of NCBI BLAST revealed that Cs cMDH shared 88%-93% of amino acid sequence identity with other cMDH from different higher plants. According to the multiple sequence alignment based on the three dimensional structure of protein, Cs cMDH was predicted to be a dimer with thirteen β sheet and thirteen α helix of each subunit. Cs cMDH contains typical fingerprint sequence (G12AAGQIG18) as all MDHs. The amino acid D43 in Cs cMDH is conserved in all NAD MDHs. Cs cMDH also has some conserved sequence units homologous to other NAD MDHs, such as NAD+ binding sites, catalytic motif and substrate binding sites. Moreover, Cs cMDH contains six Cys which are highly conserved in all plant NAD cMDHs. Therefore, Cs cMDH was inferred to be NAD dependent cMDH. The present study may provide the fundament for the further functional characterization of Cs cMDH.     

Purification and sequence determination of bovine atrial natriuretic factor

We report the purification and the sequence determination of bovine atrial natriuretic factor (ANF) in acid extracts of bovine atrial appendages. The monitoring of the activity along the purification steps was performed with a radio-receptor assay using bovine adrenal cortex membranes sites and 125I ANF. Bovine ANF was separated by carboxymethyl agarose gel chromatography from catecholamines and major protein contaminants. It behaved as a 3 K dalton peptide on Sephadex G-50. The active fractions were then subjected to high performance liquid chromatography (HPLC) using a sulfopropyl cation exchange column. Subsequent purification steps by reverse phase mode on Ultrapore RPSC, Vydac TP 218 and uBondapak using acetonitrile gradients led to the obtention of a pure fraction which amino acid sequence was identical to that for human ANF. This confirms the high degree of homology of ANF structure among mammalian species and advocates the use of the radio-receptor assay based on bovine adrenal receptor for measuring human ANF.     

家蚕核糖体蛋白L7基因cDNA序列的克隆和分析

为了研究家蚕孤雌生殖的调节机制,应用二维凝胶电泳(2DE)技术分离正常生殖的家蚕卵与孤雌生殖家蚕卵的差异蛋白质,在蛋白质水平上筛选与家蚕孤雌生殖过程相关的重要蛋白质.利用MALDI-TOF-TOF MS分析这些差异蛋白,获得了大量小肽的序列特征.BLAST搜索本实验室构建的cDNA文库,获得了1个与家蚕孤雌生殖相关的核糖体蛋白L7基因.根据已有的cDNA文库,采用RACE方法克隆得到该核糖体蛋白基因的全长cDNA.利用生物信息学的方法和工具,对这个基因在核酸水平和蛋白质水平分别作了详细的分析和讨论并进行蛋白结构预测.结果表明,核糖体L7基因的cDNA全长为858 bp,编码区包含6个外显子,共编码268个氨基酸残基,蛋白的疏水性平均值为-0.586,分子量大小为30 kD,极性的最大值为 39.616,最小值为0.451,等电点为10.52.分子系统分析显示,该蛋白与Apis, Lysiphlebus 和Meladema中的核糖体蛋白L7具有较高的同源性.     

Purification and N-terminal amino acid sequence of proliferating cell nuclear antigen (PCNA)/cyclin and development of ELISA for anti-PCNA antibodies

Proliferating cell nuclear antigen (PCNA), also called cyclin, was purified from PBS extract of rabbit thymus by using a combination of ammonium sulfate fractionation, DEAE-Sephacel, HPLC ion exchange, and HPLC gel filtration column chromatography. PCNA was purified more than 600 times and was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and immunoblotting. SDS-PAGE showed that a 36 kD protein was selectively isolated in this purification process, and this protein was identified as PCNA by immunoblotting. Other previously identified nuclear antigens, Sm, nRNP, SS-A/Ro, SS-B/La, histone, and DNA, were not detected in this preparation by counterimmunoelectrophoresis and enzyme-linked immunosorbent assay (ELISA). Purified PCNA was used as an antigen to develop ELISA for rapid and specific detection of anti-PCNA in human sera. For further purification, the 36 kD band was electrophoretically eluted from SDS gel slices. The amino acid composition and the first 25 residues from the N-terminus of the protein were determined by using electroeluted PCNA. This amino acid sequence was found to be unique and showed little sequence homology with existent proteins in the protein identification resources databank.     

Purification and characterization of rat hepatic microsomal low molecular weight fatty acid ethyl ester synthase and its relationship to carboxylesterases.

We reported purification of a high molecular weight (HMW) (ca. 180 kD) and a low molecular weight (LMW) (ca. 60 kD) protein fractions from digitonized rat liver microsomes using ammonium sulfate precipitation followed by ion exchange and gel filtration column chromatography. Both fractions expressed fatty acid ethyl ester (FAEE) synthase as well as p-nitrophenyl acetate (PNPA)-hydrolyzing (esterase) activities. The HMW fraction was found to be a trimer with subunit molecular weight ca. 60 kD and structurally and functionally similar to rat hepatic microsomal carboxylesterase (CE, pI 6.1) and adipose tissue FAEE synthase. In this article, we report further purification and characterization of the LMW (minor) fraction expressing FAEE synthase activity and its structural and functional relationship to hepatic microsomal CEs. Using isoelectric focusing (IEF) followed by gel filtration-high-performance liquid chromatography (GF-HPLC), five proteins were purified, which expressed FAEE synthase as well as PNPA-hydrolyzing activity. The isoelectric point values of 6.5, 5.8, 5.6, 5.3, and 5.0 were found for the purified LMW proteins by IEF and each showed a peak corresponding to ca. 60 kD molecular weight by GF-HPLC, which expressed FAEE synthase as well as PNPA-hydrolyzing activity. Sodium dodecyl sulfate-polyacrylamide gel elecrophoresis (SDS-PAGE) analysis of the GF-HPLC purified LMW proteins revealed that these proteins are monomers (ca. 60 kD). All the purified LMW proteins cross-reacted with antibodies to rat adipose tissue FAEE synthase. Coelution of PNPA-hydrolyzing and FAEE synthase activity at each step of purification and cross-reactivity with rat adipose tissue FAEE synthase antibodies suggest that the purified proteins are related to various hepatic microsomal CEs. This conclusion is further supported by the homology of N-terminal amino acid sequence of the purified LMW proteins to various hepatic microsomal CEs and protease precursors. Therefore, LMW FAEE synthase activity most probably is expressed by various isozymes of hepatic microsomal CEs, which are also involved in the biotransformation of xenobiotic alcohols and amines.     

苦瓜叶提取物对美洲斑潜蝇取食和产卵行为的抑制作用

美洲斑潜蝇是危害蔬菜、观赏植物的重大害虫之一.苦瓜叶乙醇提取物(浓度为2000～4000 μg·ml^-1)对美洲斑潜蝇成虫的取食和产卵都具有较强的抑制作用.用环己烷、乙酸乙酯、正丁醇和水依次对乙醇提取物进行萃取,并测试了4种萃取物对美洲斑潜蝇成虫取食和产卵的抑制作用.结果表明: 环己烷、乙酸乙酯、正丁醇和水萃取物在浓度为1000 μg·ml^-1时,处理后2 d对美洲斑潜蝇成虫的拒食率分别是11.08%、34.89%、22.99%和 0,产卵抑制率分别是0、30.91%、6.45%和 0.其中,乙酸乙酯萃取物的活性最强,当其浓度为4000 μg·ml^-1时,处理后2 d对美洲斑潜蝇成虫的拒食率和产卵忌避率分别为70.95％ 和69.49％.乙酸乙酯萃取物经硅胶柱层析分离得到(19S,23E)-5β,19-环氧-19-甲氧葫芦素-6,23-二烯-3β,25-二醇 (化合物1)、(19R,23E)-5β,19-环氧-19-甲氧葫芦素-6,23-二烯-3β,25-二醇(化合物2) 和3β,7β,25-三羟基葫芦素-5,23-二烯-19-醛缩-3-O-β-D-吡喃葡糖苷（化合物3）,3种化合物在供试的浓度（100～400 μg·ml^-1）条件下对美洲斑潜蝇的取食和产卵行为都有明显的抑制作用.在400μg·ml^-1浓度时,化合物1、化合物2和化合物3对美洲斑潜蝇成虫的拒食率分别是66.89%、53.53%和78.02%,产卵抑制率分别是76.32%、58.36%和78.36%.