名贵月季品种微繁及工艺研究

研究以名贵月季品种“落霞”、“墨红”、“和平”、“金背大红”等为试材,以ＭＳ基本培养基附加不同浓度的６－ＢＡ、ＮＡＡ,以诱导腋芽增殖为微繁途径。结果表明：无菌外植体的建立培养基为ＭＳ＋６－ＢＡＯ．５－２＋ＮＡＡＯ．０５－０．１＋Ｖｃ１００;芽增殖培养基为ＭＳ十ＢＡ１＋ＮＡＡ０．０５,在此培养基上繁殖系数为５．５;生根培养基为ＭＳ＋ＩＡＡ１＋ＩＢＡ１＋ＮＡＡ０．１－肌醇,生根率在９５％左右。生根苗移栽成活率在８５％左右。同时对繁殖工艺流程、成本、商品苗产率等问题进行了讨论,给出在繁殖系数为Ｆ、生根数为ｂ时,有效繁殖系数ｆ＝Ｆ—ｂ,试管苗实际增殖倍数Ｎｎ＝（Ｆ—ｂ）（ｎ－１）·Ｆ、生根苗数Ｒ１－ｎ＝ｆ－１;当生根率为ｒ１,移栽成活率为ｒ２,则商品苗产率为Ｃ＝ｒ１·ｒ２·Ｒｎ＝ｒ１·ｒ２·ｂ（ｆ－１）／（ｆ－１）     

Ca^2＋敏感性微电极在心肌胞浆Ca^2＋活度检测中的应用

改进的中性载体Ｃａ２＋敏感性微电极（Ｃａ－ＩＳＥ）在尖端直径为０．４—０．８μｍ时仍具有良好特性,可用于心肌胞浆Ｃａ２＋活度（αＣａｉ）的检测。测得豚鼠右心乳头肌、狗心室肌和浦肯野纤维静息时分别为０．１９±０．０１（ｎ＝２２）,０．２０±０．０２（ｎ＝１１）和０．４６±０．０７（ｎ＝１３）μｍｏｌ·Ｌ－１。毒毛旋花苷Ｇ３μｍｏｌ·Ｌ－１使静态及动态心肌分别增高０．１８±０．０２和６．６９±２．０９μｍｏｌ·Ｌ－１（ｎ＝２２）,并出现触发活动（ＴＡ）。１００μｍｏｌ·Ｌ－１蝙蝠葛碱可抑制毒毛旋花苷Ｇ引起的增高,同时使其ＴＡ消失。表明Ｃａ－ＩＳＥ技术可用于心肌组织ＴＡ与的同步检测。     

山东10种植物的核型分析

对山东１０ 种植物进行了核型分析。茴茴蒜（ Ｒａｎｕｎｃｕｌｕｓｃｈｉｎｅｎｓｉｓ Ｂｇｅ－） 染色体数目２ｎ ＝１６ , 核型公式Ｋ（２ｎ） ＝ ２ｘ ＝ １６ ＝ ２ Ｍ ＋ ２ｍ ＋ ２ｓｍ ＋ １０ｓｔ, “３Ａ”类型; 五脉地椒（ Ｔｈｙｍｕｓｑｕｉｎｑｕｅｃｏｓｔａｔｕｓ Ｃｅｌａｋ－） 染色体数目２ｎ＝ ２６ , 核型公式Ｋ （２ｎ） ＝ ２ｘ＝ ２６ ＝ ８ Ｍ ＋ １８ｍ , “１Ａ”类型; 蛇床（ Ｃｎｉｄｉｕｍ ｍｏｎｎｉｅｒｉ（Ｌ－） Ｃｕｓｓ－） 染色体数目２ｎ＝ ２０ , 核型公式Ｋ （２ｎ） ＝ ２ｘ＝ ２０ ＝ ２Ｍ＋ １６ｍ ＋ ２ｓｍ , “２Ｂ”类型; 波斯菊（ Ｃｏｓｍｏｓ ｂｉｐｉｎｎａｔｕｓ Ｃａｖ－） 染色体数目２ｎ ＝ ２４ , 核型公式Ｋ（２ｎ） ＝ ２ｘ ＝ ２４ ＝ １６ｍ ＋ ２ｍ （ｓａｔ） ＋ ６ｓｍ , “２Ａ”类型; 白车轴草（ Ｔｒｉｆｏｌｉｕｍ ｒｅｐｅｎｓ Ｌ－） 染色体数目２ｎ＝ ３２ , 核型公式Ｋ （２ｎ） ＝ ４ｘ ＝ ３２ ＝ ３２ｍ , “１Ａ”类型; 铁苋菜（ Ａｃａｌｙｐｈａ ａｕｓｔｒａｌｉｓ Ｌ－）染色体数目２ｎ ＝ ３２ , 核型公式Ｋ （２ｎ） ＝ ２ｘ＝ ３２ ＝ ３２ｍ , “１Ｂ”类型; 地构叶（ Ｓｐｅｒａｎｓｋｉａ ｔ?     

日本血吸虫雄性成虫的细胞电活动特征的研究

应用玻璃微电极的电生理实验技术,研究日本血吸虫雄性成虫的细胞电活动。结果显示：日本血吸虫雄性成虫皮层细胞膜电位为－４７±５． ６ｍＶ（Ｘ±ＳＥ;ｎ＝１０３）;肌细胞膜电位为－３０．２±４．３ｍＶ（Ｘ±ＳＥ;ｎ＝１２６）．肌细胞可记录到自发放电活动,电位去极化幅值为９—２８ｍＶ。微电极记录的部分细胞（皮层细胞 ｎ＝２５;肌细胞 ｎ＝２２）用辣根过氧化酶（Ｈｏｒｅｒａｄｉｓｈ ｐｅｒｏｘｉｄａｓｅ,ＨＲＰ）标记,进行了细胞组织学鉴定．     

尖锐湿疣患者皮损中白介素2基因表达的研究

为探讨Ｔｈ１ 反应如白介素２ （ＩＬ－２） 产生在尖锐湿疣（ＣＡ） 发病及消退中的作用。本实验采用逆转录——聚合酶链反应（ＲＴ－ＰＣＲ） 技术检测了ＣＡ患者皮损组织ＩＬ－２ 的基因表达, 实验分为三组： 正常对照组（ｎ＝ １０）, 单纯病例组（ｎ＝ １８） 及γ－ 干扰素（ＩＦＮ－γ） 诱导组（ｎ＝ ６）。结果发现正常皮肤组织未检测到ＩＬ－２ ｍ ＲＮＡ, 在１８ 例单纯病例的ＣＡ患者有２ 例皮损ＩＬ－２ ｍ ＲＮＡ阳性, ６ 例ＣＡ患者注射ＩＦＮ－γ前局部皮损未检测到ＩＬ－２ ｍ ＲＮＡ, 而在皮损内注射ＩＦＮ－γ７２ 小时后有４ 例阳性。研究结果提示了ＩＦＮ－γ可诱导Ｔｈ１ 应答, Ｔｈ１ 应答在抵抗人类乳头瘤病毒（ＨＰＶ） 感染及清除ＨＰＶ中可能起着重要作用, 为临床应用ＩＬ－２ 及ＩＦＮ－γ治疗ＣＡ提供了理论依据。     

免疫组织化学染色定量方法研究（Ⅲ）

本文对免疫组织化学染色反应的定量方法进行了研究,导出阳性单位（ＰＵ）测算新公式。根据测试区域Ａ的灰度级ＧＡ和面积（ｍ＋ｎ）及阳性反应产物α相的灰度级Ｇα和面积ｎ（或背景面积ｍ）即可求得ＰＵ。公式如下：ＰＵ＝１００×｜Ｇα－ＧＡ｜／（ＡＡβ·Ｇｍａｘ）＝１００×｜Ｇα－ＧＡ｜／［（１－ＡＡα）·ｍａｘ］。式中ＡＡα＝ｎ／（ｍ＋ｎ）,ＡＡβ＝ｍ／（ｍ＋ｎ）,Ｇｍａｘ为测试仪器的最大灰度分级。本法灰度测试无需考虑灰度设定方法,只需在同一灰度设定条件下测试即可。本法还可用于其它组织化学、细胞化学和原位分子杂交反应显色程度定量。     

半夏脱毒与快繁技术研究进展

半夏是我国传统中药材，长期无性繁殖导致病毒积累对半夏产量和品质造成了严重影响。由于半夏茎尖病毒积累少，利用半夏茎尖脱毒快繁技术可有效解决病毒害严重的问题。本研究从半夏主要病毒种类、脱毒方法、组培快繁和病毒检测等方面对半夏脱毒与快繁技术进行综述，以期为半夏脱毒快繁体系的建立提供参考。     

深红蔓绿绒的组织培养与快速繁殖

１　植物名称　深红蔓绿绒（Ｐｈｉｌｏｄｅｎｄｒｏｎｍａｎｄａｉａｎｕｍ“ＲｏｙａｌＱｕｅｅｎ”）。２　材料类别　顶芽、侧芽。３　培养条件　以ＭＳ为基本培养基。（１）芽体启动培养基：ＭＳ＋６ＢＡ２ｍｇ·Ｌ－１（单位下同）＋ＮＡＡ０．０１;（２）不定芽增殖培养基：ＭＳ＋６ＢＡ３～４＋ＮＡＡ０．１;（３）生根培养基：１／２ＭＳ＋６ＢＡ０．５＋ＩＢＡ２。以上培养基均加琼脂７．５ｇ·Ｌ－１,ｐＨ值为５．８,培养室温度（２６±２）℃,光照度１０００ｌｘ,每日光照时间１２ｈ。培养基（１）与（２）中蔗糖用…     

梅花鹿甲烷能代谢规律的研究

本文应用ＫＢ－１型呼吸测热装置,结合消化、代谢试验,对梅花鹿（Ｃｅｒｖｕｓｎｉｐｐｏｎ）甲烷能代谢规律进行了研究。结果表明,梅花鹿甲烷能的产生量随其采食量的增加而增加;也随着果食后时间的推移而减少,而且减少的幅度又随采食量的增加而下降;甲烷能的产生量分别占总能食入量、消化能食入量和体增热的６．６１％、８．８３％和１０．８８％;甲烷能的产生量随着日粮蛋白质水平的提高而降低,日粮蛋白质水平每提高１个百分点,甲烷能产生量就降低５８．５８ｋＪ／ｄ;分别以总能食入量（ＧＥＩ）和干物质食入量（ＤＭＩ）为自变量所建立的甲烷能（ＣＨ４Ｅ）估计分别为：ＣＨ４Ｅ（ｋＪ／ｄ）＝０．０７ＣＥＪ（ｋＪ／ｄ）－１０１．０４（ｎ＝１２,ｒ＝０．９４４,Ｐ＜０．０１）ＣＨ４Ｅ（ｋＪ／ｄ）＝９８．７８＋１．０５ＤＭＩ（ｇ／ｄ）（ｎ＝１２,ｒ＝０．９４２,Ｐ＜０．０１）     

马蔺组织培养快繁技术体系研究

以成熟且具活力的马蔺种子为外植体,以MS为基本培养基,与不同浓度比例的2,4-D、BA、NAA、KT等植物生长调节剂构成愈伤组织诱导、分化、生根等培养基的组合方案,对马蔺组织培养快繁技术开展系统研究。结果表明,不同植物生长调节剂组合的培养基对愈伤组织的诱导率有显著影响,MS+2,4-D 4 mg·L^-1+BA2 mg·L^-1、MS+2,4-D 4 mg·L^-1+BA5 mg·L^-1和MS+2,4-D 2 mg·L^-1+KT1.5 mg·L^-1为最佳诱导培养基,诱导出愈率均在58%以上,显著高于其它培养基组合方案（p<0.05）;最佳分化培养基为MS+BA4 mg·L^-1和MS+BA1 mg·L^-1+NAA0.15 mg·L^-1,绿苗分化率高达100%,生长势好,状态叶和分化芽丛质量好;适宜继代增殖培养基为MS+BA2 mg·L^-1+NAA0.1 mg·L^-1、MS+BA1 mg·L^-1+NAA0.2 mg·L^-1;1/2MS为最适宜的生根培养基,1/2MS+IBA0.5 mg·L^-1、1/2MS+IBA0.5 mg·L^-1+NAA0.5 mg·L^-1两种组合也相对较好;试管苗不需炼苗可直接出瓶移栽于V_田土∶V_河沙=2∶1的土壤基质,成活率在95%以上。从而为马蔺提供了一套从“成熟种胚—诱导愈伤组织—绿苗分化—继代增殖—生根—试管苗移栽”等整个过程中各环节的最佳培养基和操作规程的组培快繁体系。     

野生石菖蒲、水杨梅的调查引种及驯化栽培研究

调查了野生石菖蒲、水杨梅的生态环境和生物学特性,引种石菖蒲进行不同季节的分株繁殖试验及栽培试验,引种水杨梅进行扦插繁殖试验,基本掌握了石菖蒲、水杨梅的生物学特性和快繁技术。     

The devil's in the details: genetic and phenotypic divergence between artificial and native populations of the endangered pupfish (Cyprinodon diabolis)

Propagation of threatened or endangered species in artificial habitats is a common strategy for reducing the probability of extinction by demographic or stochastic forces. Differential selection, founder effects and genetic drift can conspire to cause artificial populations to differ irreversibly from native populations for characters important for fitness, thereby compromising conservation efforts. Here we show that artificial propagation of the endangered Devil's Hole pupfish Cyprinodon diabolis resulted in rapid divergence for phenotypic and genetic characteristics despite attempts to replicate key characteristics of the species' native habitat when designing the artificial environments. Although differences in behavior and morphology between the native pool population and the two artificial pools may reflect phenotypic plasticity, the results underscore the need to monitor and control (to the extent possible) closely the evolutionary process when propagating native species in artificial pools for multiple generations.     

Assessment of the Mulder and Van Doorn kinetic procedure and rapid centrifugal analysis of UDP-glucuronosyltransferase activities

The optimal experimental conditions of the enzyme assay described by Mulder and Van Doorn (1975, Biochem J. 151, 131-140) for the measurement of UDP-glucuronosyltransferase activities were tested towards structurally different aglycones. This assessment of this assay revealed that addition of Triton X-100 as enzyme activator was necessary because of its apparent inhibitory effects on interfering reactions. Under these conditions, accordance of the data with results published in the literature was obtained. We present for the first time an UDP-glucuronosyltransferase assay adapted on a fast analyser centrifuge which allows a rapid and sensitive measurement of enzyme activity that is very useful for kinetic constant determination, without consuming a large volume of reagents.     

铁皮石斛快速繁殖和离体种质保存的研究

对铁皮石斛种子发芽、原球茎增殖、丛芽分化和壮苗培育进行了试验、观察和分析,研究了培养基、植物激素、光强和添加剂等对其分化和生长的影响。结果显示种子在1/2MS+蔗糖2%的培养基上,30d萌发95%以上。原球茎在1/2MS+椰子汁25%+蔗糖3%的培养基上,45~60d原球茎增殖速度可达1∶10。丛芽分化较适宜的培养基为1/2MS+BA2mg·L-1+NAA0.2mg·L-1+IBA0.1mg·L-1+蔗糖3%,45~60d芽丛增殖速度为1∶4~5。试管苗在MS+香蕉泥20%+蔗糖2%培养基上,大约60d苗快速长高,茎粗壮且根系发达。离体保存材料可采用试管丛芽和原球茎两种方式,以保持其遗传多样性。保存方法是在15℃左右条件下,保存离体材料,继代间隔期为12~18个月;也可以采用室温保存,在1/2MS+蔗糖1%培养基上,继代间隔期可延长至10~12个月。     

蕨类植物孢子萌发及原叶体发育的观察

以腐叶土为培养基质,对21种蕨类植物进行了孢子萌发和原叶体发育的研究,结果表明：①不同时期播种的同种蕨类的孢子,发育出原叶体和幼孢子体所历经的时间长短不同;②孢子萌发和配子体生长发育的适宜温度约为15～24℃;⑨稀有蕨类的孢子萌发率低,而在野外能形成较大种群的蕨类的孢子萌发率高;④用GA3处理孢子可以促进萌发;⑤当原叶体上长出幼孢子体时,原叶体由大变小,由绿变黄,21种蕨类的原叶体都在幼孢子体上长出第3片叶时消失;⑥幼孢子体上长出的第1、2片叶在形态上与以后长出的叶不同;⑦孢子萌发需要光;⑧1片原叶体尽管有多个颈卵器,但仅发育出1株幼孢子体;⑨利用腐叶土进行蕨类孢子繁殖是一种经济实用的繁殖方法。     

Lipid Peroxidation. Definition of Experimental Conditions for Selective Study of the Propagation and Termination Phases

To find experimental conditions to selectively study the propagation phase of lipoperoxidation we studied the lipoperoxidation, catalyzed by FeCl₂, of liposomes in a buffering condition where Fe²⁺ autoxidation and oxygen active species generation does not occur. Liposomes from egg yolk phosphatidylcholine. prepared by vortex mixing, do not oxidize Fe²⁺: on the contrary they oxidize Fe²⁺ when prepared by ultrasonic irradiation. Dimyristoyl phosphatidylcholine liposomes prepared by ultrasonic irradiation do not oxidize Fe²⁺. During sonication polyunsaturated fatty acid residues autoxidize and lipid hydroperoxides (LOOH) are generated. Only when LOOH are present in the liposimes Fe²⁺ oxidizes and its rate of oxidation depends on the amount of LOOH in the assay. The reaction results in the generation of both LOOH and thiobarbituric acid reactive material (TBAR): it is inhibited by butylated hydroxytoluene and has a acidic pH optimum; it is not inhibited by catalase and OH' scavengers. The reaction studied. thus, appears to be the chain branching and propagation phase of lipoperoxidation. When we studied the dependence of Fe²⁺ oxidation, LOOH and TBAR generation on FeCl₂ concentration, we observed that at high FeCl₂ concentrations the termination phase of lipoperoxidation was prevalent. Thus. by selecting the appropriate FeCl₂ concentration the proposed experimental system allows study of either the propagation or the termination phase of lipoperoxidation.     

Lipid Peroxidation. Definition of Experimental Conditions for Selective Study of the Propagation and Termination Phases

To find experimental conditions to selectively study the propagation phase of lipoperoxidation we studied the lipoperoxidation, catalyzed by FeCl₂, of liposomes in a buffering condition where Fe²⁺ autoxidation and oxygen active species generation does not occur. Liposomes from egg yolk phosphatidylcholine. prepared by vortex mixing, do not oxidize Fe²⁺: on the contrary they oxidize Fe²⁺ when prepared by ultrasonic irradiation. Dimyristoyl phosphatidylcholine liposomes prepared by ultrasonic irradiation do not oxidize Fe²⁺. During sonication polyunsaturated fatty acid residues autoxidize and lipid hydroperoxides (LOOH) are generated. Only when LOOH are present in the liposimes Fe²⁺ oxidizes and its rate of oxidation depends on the amount of LOOH in the assay. The reaction results in the generation of both LOOH and thiobarbituric acid reactive material (TBAR): it is inhibited by butylated hydroxytoluene and has a acidic pH optimum; it is not inhibited by catalase and OH' scavengers. The reaction studied. thus, appears to be the chain branching and propagation phase of lipoperoxidation. When we studied the dependence of Fe²⁺ oxidation, LOOH and TBAR generation on FeCl₂ concentration, we observed that at high FeCl₂ concentrations the termination phase of lipoperoxidation was prevalent. Thus. by selecting the appropriate FeCl₂ concentration the proposed experimental system allows study of either the propagation or the termination phase of lipoperoxidation.     

城市化过程中森林meta种群结构及动态分析

采用样地每木调查法,通过丰富度、均匀度、多样性、层次结构复杂性和直径结构复杂性等指数进行分析比较,研究了快速城市化过程中深圳市不同立地等级黄牛木meta种群结构。结果表明：黄牛木群落以黄牛木[Cratoxylum cochinchinense（Lour．）Blume]和豹皮樟[Litsearotundifolia var．oblongifolia（Nees）Allen]两物种紧密组合为基本特征,立地等级越高,物种竞争力越强。立地条件好的黄牛木群落物种丰富度、均匀度和多样性比立地条件差的分别高1．58～1．85倍、0．67～0．87倍和1．34～1．60倍,说明缀块生境变差将导致群落层次结构趋于简单,群落不稳定。受城市化影响,黄牛木meta种群在台湾相思（Acacia confusa Merr．）群落和梅叶冬青[Hex asprella（Hook．et Arn．）Champ．ex Benth．]群落中明显占据优势种地位,群落有逆向演变趋势。今后应着力保护群落上层乔木层物种,改善群落缀块生境。     

History of orchid propagation: a mirror of the history of biotechnology

Part I Orchid seeds are nearly microscopic in size. Because of that, many fanciful theories were proposed for the origin of orchids. Almost 400 years separate the time when orchid seeds were seen for the first time and the development of a practical asymbiotic method for their germination. The seeds were first observed and drawn during the sixteenth century. Seedlings were first described and illustrated in 1804. The association between orchid and fungi was observed as early as 1824, while the requirement for mycorrhiza for seed germination was established in 1899. An asymbiotic method for orchid seed germination was developed in 1921. After Knudson’s media B and C were formulated, orchids growing and hybridization became widespread. Hybrids which early growers may not have even imagined became possible. Part II A commonly held view is that Prof. Georges Morel is the sole discoverer of orchid micropropagation and that he was the first to culture an orchid shoot tip in 1960. In fact, the first in vitro orchid propagation was carried out by Dr. Gavino Rotor in 1949. Hans Thomale was the first to culture an orchid shoot tip in 1956. The methods used by Morel to culture his shoot tips were developed by others many years before he adapted them to orchids. This review also traces the history of several techniques, additives, and peculiarities (agitated liquid cultures, coconut water, banana pulp, a patent and what appears to be an empty claim) which are associated with orchid micropropagation. A summary of plant hormone history is also outlined because micropropagation could not have been developed without phytohormones.

矮生龙船花的组织培养和快速繁殖

矮生龙船花(IxoracoccineaL.)的带节茎段在MS 2,4D2.0mg/L培养基上产生大量的愈伤组织;在MS 6BA1.0mg/L NAA0.2mg/L培养基上芽的增殖系数达413,并产生少量的愈伤组织;在MS NAA0.2～2.0mg/L培养基上只产生芽而无愈伤组织形成。愈伤组织在MS 6BA0.5mg/L NAA0.5mg/L培养基上产生大量的不定芽,丛生芽在MS 6BA0.5mg/L NAA0.5mg/L培养基上生长较快并产生较多分枝,将分枝节下或切成段后在MS 6BA0.5mg/L NAA0.5mg/L培养基上能迅速生长并产生新的分枝。试管内小苗在1/2MS NAA0.5mg/L培养基上的生根壮苗效果较好。矮生龙船花试管苗成活率为935%。