隆线溞孤雌溞生殖系统的组织学

隆线孤雌的生殖系统由一对卵巢、一对输卵管和一对雌性生殖孔组成。卵巢长管状 ,管壁由结缔组织膜和单层上皮细胞构成 ,末端渐细为一短小的输卵管 ,输卵管末端为雌性生殖孔。卵子的发生是由生发区细胞向卵巢内增殖分化 ,不同成熟度的生殖细胞在管腔内排列成生殖带。根据卵母细胞细胞核的大小及卵黄的累积情况等 ,将卵子的发生划分为三个时期 :卵原细胞、卵母细胞和成熟卵子 ,其中卵母细胞的发生又可细分为三个时期 :前期、中期和后期。后期的卵母细胞含较多的卵黄颗粒 ,最后成为成熟卵子 ,排入孵育囊内形成夏卵。隆线孤雌的卵巢发育要经历五个幼龄期 ,不同的龄期 ,卵巢的形态结构不同。至第五幼龄 ,卵巢已基本发育成熟 ,准备排卵进入第一成龄     

微齿喜马拉雅低额溞的生殖与发育

对微齿喜马拉雅低额溞（Ｓｉｍｏｃｅｐｈａｌｕｓ ｈｉｍａｌａｙｅｎｓｉｓ　ｍｉｏｒｏｄｕｓ）的生殖和发育进行研究的结果表明：在２０±１℃换水条件下，喂以斜生栅藻（４０万个／ｍｌ），此　有４个幼龄、１６个成龄，平均寿命４８．７±８．９２天。平均总产仔量３６１．ｌ±２１．５个，最大生殖量在第１０龄（第６成龄）。已经证明从冬卵（受精卵）来的孤雌生殖溞在体长和产仔量上都高于其来自孤雌卵的下代孤雌　。两性生殖与降低温度有关，发生在秋季生殖高峰期水温已下降时，与食物的多少无直接关系。本种在自然界属于单周期型，它的交配行为特殊与其仰游习性相适应。文章对冬孵和孤雌卵的发育做了描述。     

隆线潘孤雌溞生殖系统的组织学

隆线溞孤雌溞的生殖系统由一对卵巢、一对输卵管和一对雌性生殖孔组成。卵巢长管状,管壁由结缔组织膜和单层上皮细胞构成,末端渐细为一短小的输卵管,输卵管末端为雌性生殖孔。卵子的发生是由生发区细胞向卵巢内增殖分化,不同成熟度的生殖细胞在管腔内排列成生殖带。根据卵母细胞细胞核的大小及卵黄的累积情况等,将卵子的发生划分为三个时期：卵原细胞、卵母细胞和成熟卵子,其中卵母细胞的发生又可细分为三个时期：前期、中期和后期。后期的卵母细胞含较多的卵黄颗粒,最后成为成熟卵子,排入孵育囊内形成夏卵。隆线溞孤雌溞的卵巢发育要经历五个幼龄期,不同的龄期,卵巢的形态结构不同。至第五幼龄,卵巢已基本发育成熟,准备排卵进入第一成龄。     

松毛虫赤眼蜂孤雌产雌品系田间控害作用研究

【目的】为明确感染Wolbachia的松毛虫赤眼蜂孤雌产雌品系对亚洲玉米螟的防治效果。【方法】2012和2013连续两年于沈阳地区玉米田间释放松毛虫赤眼蜂孤雌产雌品系和两性生殖品系。【结果】2012年孤雌产雌品系对1代亚洲玉米螟卵寄生效果为66.39%,对2代玉米螟卵寄生效果为69.53%,与对照(松毛虫赤眼蜂两性品系)相比无显著差异(分别为56%,79.73%)(P≥0.05),2013年孤雌产雌品系对1代亚洲玉米螟卵寄生效果为56.20%,对2代玉米螟卵寄生效果为82.10%,与对照相比无显著差异(分别为52.24%,75.71%)(P≥0.05)。收获前期剖杆结果表明,2012年孤雌产雌品系及对照对玉米螟的防治效果分别为22.50%、27.50%,2013年分别为38.28%、21.09%,连续两年的防治效果无显著差异(P≥0.05)。【结论】从田间试验结果可以看出,孤雌产雌松毛虫赤眼蜂品系可取得与生产用两性松毛虫赤眼蜂品系同期的防治效果,且孤雌产雌松毛虫赤眼蜂在种群增长速率、降低规模化培养成本、低密度种群下进入新生境并建立种群等方面都要优于正常松毛虫赤眼蜂品系,因此其具有很好的生防应用效果。     

温度和种间竞争对大型溞种群动态和两性生殖的影响

在20℃、25℃下,将大型溞和老年低额溞分别按7+3(B组),5+5(C组),3+7(D组)的组合进行混合培养,以及用单种培养(10+0(A组),0+10(E组))作为对照,研究了温度和种间竞争对大型溞种群动态和两性生殖的影响.实验结果表明:在混合培养时,大型溞对老年低额溞产生明显的竞争优势.20℃、25℃下,单种培养的老年低额溞最大种群密度分别为大型溞的2.31和1.97,而在混合培养下老年低额溞的种群密度明显低于大型溞,在实验25d后几乎全部死亡.25℃下两种溞的种群密度之间存在极显著的负相关性(C组:r=-0.508,n=30,P<0.01;D组:r=-0.483,n=30,P<0.01).在20℃、单种培养下,大型溞在首次产幼溞时即出现雄体,且种群密度与雄体密度呈显著的相关性(r=0.678,n=24,P<0.01).大型溞的最大雄体密度(106 ind.(200ml)~(-1))和最大雄体比例(36.8%)均出现在20℃、单种培养下.25℃下,大型溞在混合培养的B组和C组首次产幼溞时即出现雄体,且雄体在混合培养B组的比例达28.2%.大型溞在25℃、单种培养下没有产生卵鞍,在混合培养下总计产生66个卵鞍,其中空卵鞍占51.5%,而在20℃、混合培养下没有卵鞍产生.实验结果暗示:在较高的温度下,种间竞争刺激了大型溞雄体的产生和卵鞍的形成,高密度的雄体有助于大型溞孤雌生殖雌体向两性生殖雌体的转化.     

松毛虫赤眼蜂两性生殖品系和孤雌产雌品系在不同品种柞蚕卵中的寄生和生长发育表现

【目的】明确两性生殖品系和孤雌产雌品系松毛虫赤眼蜂Trichogramma dendrolimi在不同品种柞蚕Antheraea pernyi卵中的寄生及发育表现,为以柞蚕卵为替代寄主更好地规模化繁育赤眼蜂提供依据。【方法】测定两性生殖品系和孤雌产雌品系雌蜂在6个品种柞蚕卵［抗大(KD)、大四(DS)、高新(GX)、988(NEE)、青大(QD)和特大(TD)］上的寄生率、子代蜂窝蜂数(单窝羽化子代蜂数)和子代蜂雌性比等生物学指标,以及6个品种柞蚕卵的质量指标(单卵湿重、蛋白质含量、总糖含量和甘油三酯含量);利用主成分分析揭示柞蚕卵质量指标与赤眼蜂生物学指标间的相关性。【结果】NEE品种柞蚕卵育出的两性品系松毛虫赤眼蜂子代蜂个体显著大于除KD和QD品种以外的其他柞蚕品种卵育出的两性品系子代蜂。柞蚕品种对两性品系松毛虫赤眼蜂的寄生率、子代蜂窝蜂数和子代蜂雌性比均无显著影响。在孤雌产雌品系松毛虫赤眼蜂中,KD品种柞蚕卵育出的松毛虫赤眼蜂子代蜂窝蜂数最多,显著高于NEE和QD品种育出的子代蜂窝蜂数,但与DS, GX和TD品种育出的子代蜂窝蜂数相比无显著差异。柞蚕品种对孤雌产雌品系松毛虫赤眼蜂的寄生率和子代蜂个体大小均无显著影响。TD品种柞蚕卵的蛋白质含量最高,显著高于除GX品种以外的柞蚕品种。KD品种柞蚕卵的总糖含量和QD品种柞蚕卵的甘油三酯含量最高,均分别显著高于其余柞蚕品种。主成分分析表明,两性品系松毛虫赤眼蜂寄生率、柞蚕卵蛋白质含量和甘油三酯含量均与柞蚕卵总糖含量呈负相关;两性品系松毛虫赤眼蜂子代蜂个体大小和柞蚕卵甘油三酯含量与单卵湿重呈负相关;孤雌产雌品系松毛虫赤眼蜂寄生率和柞蚕卵甘油三酯含量与松毛虫赤眼蜂子代蜂窝蜂数、柞蚕卵总糖含量和单卵湿重呈负相关;孤雌产雌品系松毛虫赤眼蜂子代蜂个体大小和柞蚕卵总糖含量与蛋白质含量呈负相关。【结论】本研究通过筛选适宜两性生殖品系和孤雌产雌品系赤眼蜂繁育的柞蚕卵品种,初步明确了卵内主要营养指标与子代蜂生物学指标间的相关性。研究结果为利用柞蚕卵更好地规模化繁育松毛虫赤眼蜂提供依据与数据支撑。     

不同温度下松毛虫赤眼蜂孤雌产雌品系和两性生殖品系对米蛾卵的寄生功能反应

赤眼蜂部分蜂种或品系受Wolbachia侵染营孤雌产雌生殖。 通过室内试验分析了在4个恒温（20, 25, 30和35℃）下松毛虫赤眼蜂Trichogramma dendrolimi两性生殖品系和孤雌产雌品系对米蛾Corcyra cephalonica卵的寄生功能反应, 旨在比较不同温度两品系的寄生功能反应差异, 评价孤雌产雌品系在生物防治中的应用潜力。 结果表明： 松毛虫赤眼蜂两个品系对米蛾卵寄生作用均随寄主密度的增加而增大;随温度的升高松毛虫赤眼蜂两品系的功能反应类型由Ⅲ型改变为Ⅱ型。孤雌产雌品系以30℃的处置时间最短(0.0207 d), 最大日寄生量为48.31粒卵, 其次是25℃, 35℃最小;两性生殖品系以25℃的处置时间最短(0.0188 d), 最大日寄生量为53.08粒卵, 其次是30℃, 20℃最小; 松毛虫赤眼蜂两品系的寄生功能反应存在显著差异, 30℃下孤雌产雌品系为Ⅱ型功能反应而两性生殖品系为Ⅲ型。 从处置时间来看, 20℃时两品系无显著性差异(P≥0.05), 在25℃和35℃孤雌产雌品系寄生米蛾卵时花费的时间显著长于两性生殖品系(P<0.05), 而30℃却相反。 可见, 寄主密度、 温度和Wolbachia影响松毛虫赤眼蜂功能反应。     

温度对发头裸腹溞生殖能力的影响

在实验室培养条件下饲以充足食物,对不同温度下发头裸腹溞(Moina irrasa)的最大生殖能力进行了研究。结果表明：在5个不同温度（(15±1)℃、(20±1)℃、(25±1)℃、(30±1)℃、(35±1)℃）条件下,发头裸腹溞最大生殖个体的体长可达1.93mm;性成熟所需的时间分别为：4.0d、2.36d、1.40d、1.31d和1.0d;各成龄期平均产仔量为：(24.78±4.29)个、(19.1±2.42)个、(26.25±5.71)个、(27.62±2.72)个和(19.47±3.29)个;平均累计产仔量则为：(87±26)个、(159±39.5)个、(239±21.9)个、(130.9±36.1)个、(81.6±17.0)个。发头裸腹溞的最适生殖温度在25－30℃之间,25℃时其累计生殖量最大,为(239±21.9)个。生殖的极限温度最高约为38℃,生活的临界温度最高在40℃。温度低于11℃时发头裸腹溞已不适合进行孤雌生殖。在不同温度条件下,发头裸腹溞性成熟所需的时间与水温的关系可用回归方程表示为：h=7231.4t-1.6167。本文亦对同属中几个相近种的生殖能力及相关生物学现象进行了探讨。     

水稻红莲型细胞质雄性不育系小孢子不同发育时期花药总蛋白质比较分析

采用双向凝胶电泳对水稻红莲型细胞质雄性不育的不育系小孢子发育单核期和二核期花药总蛋白进行了分离,通过银染显色,获得了分辨率和重复性较好的双向电泳图谱,且单核期和二核期花药总蛋白质在双向电泳胶上分布的图谱十分相似。PDQuest 2DE图像分析软件在等电点(pI)3.0~10.0、分子量(M.W.)9.0~98.0 kD之间可识别约1 800个蛋白质点。比较分析发现单核期和二核期花药中共有241个差异表达的蛋白质点,其中仅在单核期中表达的点数为125,仅在二核期中表达的为13点;表现为表达量差异的105点,其中在二核期表达下调的点数为70点,表达上调的为33点。还对蛋白质点集中的区域(pI 4.5~8.0,M.W.25.0~70.0 kD)中的41个差异蛋白质点进行了分子量和等电点分析。     

孤雌产雌生殖品系松毛虫赤眼蜂产卵强度 对Wolbachia诱导的其生殖表型的影响

【目的】松毛虫赤眼蜂Trichogramma dendrolimi是一种用于鳞翅目害虫生物防治的重要卵期寄生蜂。本研究旨在明确孤雌产雌生殖品系松毛虫赤眼蜂的产卵强度对其体内Wolbachia滴度及Wolbachia诱导的孤雌产雌生殖表型的影响。【方法】在室内调查了3个处理组松毛虫赤眼蜂雌蜂不同产卵强度(每日仅1 h供寄主卵、隔日24 h供寄主卵和持续供寄主卵)对其生物学指标包括7 d内逐日子代雄性比、逐日产卵量、累积子代雄性比和累积产卵量的影响;采用实时荧光定量PCR方法检测未产卵雌蜂(对照)以及每日仅1 h供寄主卵和持续供寄主卵的雌蜂体内Wolbachia滴度(wsp基因拷贝数)。【结果】持续供寄主卵的雌蜂累积子代雄性比显著高于每日仅1 h供寄主卵,但与隔日24 h供寄主卵相比无显著差异。3个处理组雌蜂逐日子代雄性比随日龄的增加均显著上升,其中持续供寄主卵的处理组的上升幅度最高。持续供寄主卵的雌蜂累计产卵量显著高于每日仅1 h供寄主卵和隔日24 h供寄主卵。3个处理组雌蜂逐日产卵量随日龄的增加而显著下降,其中持续供寄主卵的处理组的下降幅度最高。未产卵的雌蜂体内Wolbachia滴度显著高于持续提供寄主卵的雌蜂体内的滴度,但与每日仅1 h供寄主卵的雌蜂体内的滴度相比无显著差异。【结论】结果说明,当松毛虫赤眼蜂雌蜂产卵不受限制时,Wolbachia滴度减少,宿主孤雌产雌表型减弱;而限制雌蜂产卵有助于维持Wolbachia滴度和宿主孤雌产雌表型。研究结果为认识Wolbachia与宿主赤眼蜂之间的互作以及应用孤雌产雌生殖品系松毛虫赤眼蜂防控害虫提供一定的参考。     

黄瓜器官特异蛋白的研究

利用 SDS单向电泳对黄瓜 ( Cucumissativus L .)的根、茎、叶、花萼、花冠、雄蕊、花柱和子房的可溶性蛋白进行了分析和比较。检测到花冠中的 2 3.5 k D和 33.0 k D,雄蕊中的 1 8.8k D、2 8.5 k D、31 .0 k D、37.0 k D和 39.0 k D,花柱中的 4 5 .0 k D及子房中的 32 .5 k D蛋白 ,分别为各自器官中的器官特异蛋白质。对花冠、雄蕊、花柱和子房的可溶性蛋白的 IEF- SDS双向电泳分析也确定了相应于 SDS单向电泳上特异蛋白带的蛋白质斑点。而且相应于 SDS单向电泳上的一条带 ,在 IEF- SDS双向电泳上可能是一个以上的分子量相同而等电点不同的几个蛋白质斑点。各种器官的蛋白质含量以雄蕊为最高、花萼为最低。     

油松雌性不育系的POD同工酶和蛋白质多肽分析

用聚丙烯酰胺凝胶电泳技术分析了油松雌性不育系和可育系雌配子体发育关键时期的POD和蛋白质多肽的变化。结果表明不育系POD同工酶在雌配子体处于几十个游离核时期活性较高,在雌配子体游离核停止分裂期活性降低,雌配子明显败育的后期,该酶的活性又有所增强。不育系的POD同工酶谱与可育系存在差异,出现了Rf值分别为0.39、0.77两条特异谱带,Rf为0.77的谱带不仅稳定而且表达量很高,Rf值为0.56的谱带表达量明显低于可育株。蛋白质多肽的分析结果表明不育系中存在分子量为18．7kD的特异蛋白质多肽,分子量为38．3kD的蛋白质多肽表达量明显低于可育系。     

Female specific proteins in Triatoma infestans haemolymph

The presence of female specific proteins in triatoma infestans haemolymph, as well as the relationship between the female specific proteins and egg proteins, were analysed. At the same time, the presence of specific female proteins in different instars was studied. Cellulose acetate electrophoresis, polyacrylamide gel electrophoresis, and immunochemical methods were used.No differences between immature female and male haemolymph were established. Female haemolymph obtained from insects with ovary development revealed quantitative differences, with cellulose acetate, with respect to the control males. With polyacrylamide gel electrophoresis, one component that is not detected in control males was detected in mature female haemolymph. With immunochemical assays, at least two antigenic components that were not observed in male haemolymph were detected.Egg extract showed, with cellulose acetate, two bands with a mobility similar to that of the proteins increased in the haemolymph of the mature female; with polyacrylamide gel, two major bands with a mobility similar to that of the specific female haemolymph protein were detected. Egg extract contains at least two components demonstrated by double-diffusion assays and three components by immunoelectrophoresis, with immunological identity to specific mature female haemolymph proteins.The extract obtained from recently hatched insects revealed two components with immunological identity to specific female proteins. Haemolymph from first, second, third, fourth and fifth instars do not appear to contain any femalespecific haemolymph protein.     

The Floral Specific Proteins of Cucumber

Soluble proteins extracted from various organs of cucumber (Cucurnis sativus L. ) were analyzed using the technique of SDS one dimensional gel electrophoresis. The majority of the proteins were expressed in more than one organ, while those specific to only one organ were comparatively rare. Only two of all the proteins analized appeared to be truely organspecific. A 40.0 kD protein and a 30.8 kD protein were observed only in extracts of reproductive organs stamen and ovary. Some proteins were specific only to certain reproductive organ. They are 35.0 kD and 34.0 kD in sepal, 18. 8 kD, 28.5 kD, 31.0 kD, 37.0 kD and 39.0 kD in stamen, 45.0 kD in style with stigma and 32.5 kD in ovary. IEF-SDS two-dimensional'electrophoresis showed that many of the one-dimensional gel bands represented several proteins dots in the 2-D and that some of them were unique to an organ-type of the flower. Protein analysis of the various organs showed that stamens contained the greatest amount and petals the least amount of protein.     

家蚕精巢蛋白质的双向电泳及质谱分析

精巢是雄性家蚕Bombyx mori的生殖腺,它的主要功能是产生精子,全面检测和鉴定精巢器官的蛋白分布将为分析家蚕雄性个体的发育和繁殖奠定基础。本研究利用双向聚丙烯酰胺凝胶电泳和蛋白硝酸银染色技术对家蚕5龄第5天幼虫的精巢组织进行了蛋白检测,利用基质辅助激光解析质量飞行时间质谱（MALDI-TOF-MS）对表达量较高的蛋白点进行了肽质量指纹图谱鉴定。结果表明：家蚕精巢蛋白质可以检测出1 000个以上的蛋白点,这些蛋白点主要集中在分子量为15～90 kD区域,等电点3.5～9之间,其中60个蛋白点得到了成功鉴定,按照已知或推测的蛋白功能,将其分为8类,包括：细胞骨架和细胞结构蛋白,膜蛋白或信号相关蛋白,大量应激反应蛋白（伴侣蛋白）,线粒体和能量产生相关蛋白,转录调控和翻译及DNA/RNA结合相关蛋白,酶和少量血液组成蛋白。其中很多蛋白可能在鞭毛形成、能量代谢及减数分裂过程中有重要作用。这些结果为进一步认识家蚕精子形成过程提供了重要的生物学信息。     

Molecular heterogeneity of Cowpea (Vigna unguiculata Fabaceae) seed storage proteins

81 wild forms and 110 cultivated cowpea,Vigna unguiculata, accessions from 21 countries of Africa were screened for variability in seed storage proteins. Total seed proteins, albumin and globulin fractions were investigated by means of sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and isoelectric focusing (IEF) of nonreduced and/or reduced samples in one- and two-dimensional procedures. The globulin fraction is heterogeneous in molecular weight and contains both legumin-like components and three to six nondisulfide-linked subunits. Three globulin subunits, with molecular weights 110, 76, and 41 kD were found to be composed of disulfide-linked polypeptides. In the nondisulfide-linked fraction, both cultivated and wild forms exhibited patterns of four types (A–D). This fraction contains polypeptide subunits of molecular weights 62, 56, and 52 kD for A type, 62, 56, 54, and 52 kD for B type, 62, 56, 52, and 50 kD for C type, and at least 62, 56, 54, 52, 50, and 49 kD for D type. These subunits present similar multiple charge forms but C and D types possess more basic specific 50 and 49 kD nondisulfide linked components. Major albumin fraction contains subunits of 94, 86, 32, and 24kD. No infraspecific variation was observed in albumin or legumin-like fractions. The discussion is focussed on the relations between genetic variability assessed by storage protein coding genes and phenotypic variability.     

Variation of Storage Proteins and Isozymes within Maize Inbred Lines

Seed storage proteins of ten maize inbred lines were investigated by sodium dodecyl sulfate polyacrylamide gel electrophoresis. In addition, fourteen isozyme loci representing nine isozyme systems were analysed. Salt-soluble protein fraction contained a large number of proteins (30 – 40 bands) of different sizes with genotypic differences among the ten inbred lines. The methionine-rich 10 kD zein showed differential expression in the ten inbred lines with different migration rates on the SDS-PAGE. This polypeptide was completely absent in the inbred line G221D. Among nine of the inbred lines, eight of 14 isozyme loci were polymorphic and six were monomorphic resulting in seven unique fingerprints.     

褐飞虱卵黄蛋白的分离及其生化特性

电泳结合不同染色方法证实, 褐飞虱Nilaparvata lugens (Stål)卵黄蛋白为一种糖脂结合蛋白,其分子量约为314 kD,由148 kD、124.5 kD和39.6 kD 3个亚基组成。免疫反应证明,卵黄蛋白只存在于生育期的雌性褐飞虱成虫体内。褐飞虱卵黄蛋白具有种的特异性,其免疫血清与白背飞虱的卵黄蛋白无交叉反应。     

Visible fluorescent detection of proteins in polyacrylamide gels without staining

2,2,2-Trichloroethanol (TCE) incorporated into polyacrylamide gels before polymerization provides fluorescent visible detection of proteins in less than 5min of total processing time. The tryptophans in proteins undergo an ultraviolet light-induced reaction with trihalocompounds to produce fluorescence in the visible range so that the protein bands can be visualized on a 300-nm transilluminator. In a previous study trichloroacetic acid or chloroform was used to stain polyacrylamide gel electrophoresis (PAGE) gels for protein visualization. This study shows that placing TCE in the gel before electrophoresis can eliminate the staining step. The gel is removed from the electrophoresis apparatus and placed on a transilluminator and then the protein bands develop their fluorescence in less than 5min. In addition to being rapid this visualization method provides detection of 0.2microg of typical globular proteins, which for some proteins is slightly more sensitive than the standard Coomassie brilliant blue (CBB) method. Integral membrane proteins, which do not stain well with CBB, are visualized well with the TCE in-gel method. After TCE in-gel visualization the same gel can then be CBB stained, allowing for complementary detection of proteins. In addition, visualization with TCE in the gel is compatible with two-dimensional PAGE, native PAGE, Western blotting, and autoradiography.     

Proteome analysis of the silkworm (Bombyx mori. L) colleterial gland during different development stages

The silkworm, Bombyx mori, colleterial gland developed very slowly until 2 days before emergence, then markedly enlarged due to the accumulation of a glue-like substances (mainly including 85% water and 11% proteins). However, the No glue (Ng) mutant female moth secreted only very little glue-like substance and laid loose eggs naturally. High-resolution two-dimensional polyacrylamide gel electrophoresis, followed by computer-assisted analysis, was used to screen the secretory region of colleterial gland protein patterns during different development stages to find quantitative and qualitative difference in protein expression during the pupae and moth stages. More than 700 protein spots were resolved in different developmental stages from the secretory region of the glands and most of the proteins were distributed in the mass range from 30 to 70 kD with pH 4-8. Through comparison and analysis, it was found that 3 proteins were only expressed in the later pupae stage (one or two days before emergence) and moth stage. Furthermore, these proteins were not expressed in the Ng mutant especially actin. There was a great variation of some protein expression volume during the development. Protein spots that changed more than 1.5-fold in expression level (relative to day 9), including 6 spots that were down-regulated and 2 spots that were up-regulated in expression were excised for identification by matrix-assisted laser desorption/ionization-time of flight mass spectrometry. Results indicated that actins that participated or regulated the exocytosis of colleterial gland and other differentially expressed proteins might be related to colleterial gland development or the secretion of a glue-like substance.