香蕉果实后熟过程中果肉软化差异的研究

对香蕉果实贮藏过程中内、外果肉相关生理生化指标及细胞结构的变化进行系统的观察分析,结果显示:(1)在贮藏初期香蕉果实内果肉的硬度小于外果肉,在贮藏过程中的同一时期,均表现出内果肉硬度小于外果肉,且内果肉硬度较外果肉先降到零;(2)在贮藏初期内果肉中多聚乳糖醛酸酶(PG)和淀粉酶的活性均高于外果肉,随着贮藏时间的延长,酶活性在内、外果肉均表现出不断增加,且这两种酶活性在内果肉中早于外果肉达到最高值,但其在内果肉中的最高值均略低于外果肉的最高值;而淀粉含量却相反,在贮藏初期内果肉中淀粉含量低于外果肉,且在贮藏过程中的降解速率高于外果肉;(3)超微结构显示,香蕉果实内果肉中淀粉粒和细胞壁结构的降解均早于外果肉.研究表明,香蕉果实的软化首先由内果肉细胞降解开始,并呈放射状向外逐步延伸.     

Competition and fruit set in the Washington navel orange

In the Washington navel orange [ Citrus sinensis (L.) Osbeck] an increase in the number of flowers results in a reduction of flower weight at anthesis and the initial fruit growth rate, and the number of developing fruitlets increases. Most of these fruitlets are shed during post-anthesis, and the final set of fruit is unrelated to the number of flowers and to the total amount of metabolites and mineral elements used up in fructification but appears to be controlled by the capacity of the tree to supply metabolites to the developing fruitlets during post-anthesis. When the number of flowers is too large, there is a reduction both in the number of initially developing fruitlets and in their growth rate. The final set of fruit is reduced through a different mechanism acting at anthesis and involving differences in mineral composition, which impairs the capacity of the fruit to act as a sink.     

香蕉果实成熟软化过程中β-D-木聚糖苷酶活性变化

β-D-木聚糖苷酶是细胞壁半纤维素中阿拉伯木聚糖和木聚糖残基降解的主要酶,对香蕉贮藏过程中果皮、果肉中β-D-木聚糖苷酶活性以及果实硬度、呼吸强度和乙烯释放量的变化进行测定分析。结果显示:β-D-木聚糖苷酶活性在果实贮藏初期的变化很小,到果实硬度开始急剧下降时迅速增加,其增加量在果皮和果肉中分别为12和22倍以上,且果肉中的酶活性大于果皮中;乙烯吸收剂处理延缓了香蕉果实呼吸和乙烯的高峰出现以及果实硬度、果肉和果皮中β-D-木聚糖苷酶活性变化的速度和幅度,但并不改变其活性的变化趋势。结果证明,β-D-木聚糖苷酶能诱导香蕉果实成熟,在果实软化中起着十分重要的作用,且其活性受乙烯的调节。     

香蕉果实成熟软化时果皮和果肉中α-L-阿拉伯呋喃糖苷酶活性的变化

阿拉伯糖是果实软化过程中变化最明显的细胞壁糖残基之一,α-L-阿拉伯呋喃糖苷酶是导致细胞壁多糖中阿拉伯糖残基降解的主要糖苷酶。为阐明该酶在香蕉果实成熟软化中的作用,实验对香蕉贮藏过程中果皮和果肉中该酶活性以及果实硬度、呼吸强度和乙烯释放量的变化进行了研究。结果表明:α-L-阿拉伯呋喃糖苷酶在果实初期的变化很小,到果实硬度开始急剧下降时达到最大,增加量达10倍以上,且果肉中的酶活性大于果皮中;乙烯吸收剂处理延缓了香蕉果实呼吸和乙烯高峰的出现时间,降低了果实硬度、果皮和果肉中α-L-阿拉伯呋喃糖苷酶活性变化的速度和幅度。以上结果表明α-L-阿拉伯呋喃糖苷酶起诱导香蕉果实成熟的作用,在果实的软化中起着十分重要的作用,且其活性受乙烯的调节。     

An experiment on Impatiens New Guinea for 11–12 year olds

The following experiment describes an easy experiment for children 11–12 years old, performed during spring in a compulsory school near Karlstad, Sweden. Four different ripe fruits were placed under flowering plants of Impatiens New Guinea (Impatiens hawkeri) for four days on a table and with plastic bags around both plants and fruits. For one of the ethylene-producing fruits, apple, the result was very clear. The plants shed many flowers and buds on the first day, due to stimulated senescence caused by ethylene. For the other ethylene-producing fruit, kiwi fruit, the result was clear but not as explicit as for apple. On the other two fruits, orange and lemon, flowers and buds were shed in the same proportion as the control plants. From these results a discussion could focus on tips on how to stimulate the ripening of unripe fruit e.g. by putting apples in the same dish. The experiment is planned in a formal scientific manner and thus stimulates discussion about how to design experiments. Very few materials are required — just flowering pot-plants, fruits and plastic bags. These are easy to buy in a garden centre or a shop. Furthermore, the experiment is cheap, it is easy to perform and it stimulates practical work.     

Polygalacturonase: a candidate gene for the soft flesh and deciduous fruit mutation in Capsicum

The soft flesh and deciduous fruit of pepper (Capsicum spp.) originated from the wild C. frutescens BG 2816 accession is a complete dominant trait controlled by the S gene. We constructed an F₂ population from a cross of BG 2816 (SS) and the bell-type C. annuum cultivar Maor (ss) and determined that S cosegregated with the tomato fruit-specific endo-polygalacturonase (PG) gene. The soft flesh and deciduous fruit phenotypes were observed together in all F₂ individuals, indicating a pleiotropic effect of PG on the two traits. We mapped S to pepper chromosome 10 in the region corresponding to that in which PG was previously mapped in tomato. Northern, RT-PCR and western analyses and enzyme activity assays, collectively, indicated that PG is not detected in green, breaker or red fruits of Maor, nor in green fruits of BG 2816. Accumulation of PG mRNA and protein was detected in the fruits of BG 2816, and it increased during ripening from breaker to red stages. The sequence analysis of partial PG cDNA isolated from BG 2816 revealed high homology (87% identity) with the tomato PG. The resemblance of the soft flesh and deciduous fruit phenotypes to PG-associated phenotypes in other fruit crops, the complete linkage between Sand PG, and the greater expression of PG in the fruits of BG 2816 than in those of Maor, all strongly indicate that PG is a candidate gene for S.     

减压处理对采后杏果实软化的生理控制效应

以串枝红杏为试材,研究了减压处理对高湿、(0±0.5)℃条件下采后杏果实生理生化变化的影响,探讨了减压处理抑制杏果实软化的生理机制。结果表明:随着贮藏时间的延长,减压和常压处理的果实硬度均逐渐下降,但同期减压处理硬度始终较高且下降的幅度小,而它们的水溶性果胶含量和相对电导率呈现持续增加的趋势,且同期减压处理值越低增加的幅度越小;减压处理的呼吸强度和多聚半乳糖醛酸酶(PG)活性峰值低且出现迟;2种处理的丙二醛(MDA)含量和脂氧合酶(LOX)活性均呈现先升后降趋势且出现峰值时间相同,但对照的峰值和升降幅度更大;常压和减压处理冷害程度不断加重,腐烂果率和失重率逐渐增大,但减压处理均明显低于同期常压处理。研究发现,减压处理能有效降低采后杏果实的呼吸强度、多聚半乳糖醛酸酶和脂氧合酶活性,维持果肉细胞的正常结构和功能,从而延缓杏果实软化衰老进程。     

Expression and import of an active cellulase from a thermophilic bacterium into the chloroplast both in vitro and in vivo

A bacterial thermostable cellulase, the endo-1,4--D-glucanase E1 from Acidothermus cellulolyticus, was imported into chloroplasts, and an active enzyme was recovered both in vitro and in vivo. Precursor fusion proteins were synthesized with E1 or its catalytic domain, CD, fused to the transit peptide of ferredoxin or ribulose-bisphosphate carboxylase activase for stromal targeting. A spacer region of 1, 5 or 15 amino acids was included carboxy to the transit peptide. The efficiency of import and processing by the stromal processing peptidase depended on the nature of the transit peptide and the passenger protein, and increased with the length of the spacer between them. Besides finding E1 or CD in the stroma, protein was arrested in the envelope during import showing that structural features of E1 and CD, along with their proximity to the transit peptide, influence translocation. The cellulose binding domain and/or serine/proline/threoline-rich linker of E1 may impede efficient import. Significantly, most precursors for E1 and CD synthesized by in vitro translation possessed endoglucanse activity that was temperature-dependent, and required the residues AGGGY at the N-terminus of E1 and CD. Furthermore, activity was detected upon import into chloroplasts. Based on the in vitro analyses, five precursor fusion proteins were selected to determine if E1 and CD would be successfully targeted to chloroplasts in vivo. In transgenic tobacco plants, E1 and CD accumulated in both the stromal and membrane fractions and, importantly, chloroplast extracts showed endoglucanase activity.     

Differential expression of expansin gene family members during growth and ripening of tomato fruit

cDNA clones encoding homologues of expansins, a class of cell wall proteins involved in cell wall modification, were isolated from various stages of growing and ripening fruit of tomato (Lycopersicon esculentum). cDNAs derived from five unique expansin genes were obtained, termed tomato Exp3 to Exp7, in addition to the previously described ripening-specific tomato Exp1 (Rose et al. (1997) Proc Natl Acad Sci USA 94: 5955–5960). Deduced amino acid sequences of tomato Exp1, Exp4 and Exp6 were highly related, whereas Exp3, Exp5 and Exp7 were more divergent. Each of the five expansin genes showed a different and characteristic pattern of mRNA expression. mRNA of Exp3 was present throughout fruit growth and ripening, with highest accumulation in green expanding and maturing fruit, and lower, declining levels during ripening. Exp4 mRNA was present only in green expanding fruit, whereas Exp5 mRNA was present in expanding fruit but had highest levels in full-size maturing green fruit and declined during the early stages of ripening. mRNAs from each of these genes were also detected in leaves, stems and flowers but not in roots. Exp6 and Exp7 mRNAs were present at much lower levels than mRNAs of the other expansin genes, and were detected only in expanding or mature green fruit. The results indicate the presence of a large and complex expansin gene family in tomato, and suggest that while the expression of several expansin genes may contribute to green fruit development, only Exp1 mRNA is present at high levels during fruit ripening.     

香蕉果实软化相关β-半乳糖苷酶基因的克隆及其表达分析

β-半乳糖苷酶（β-galactosidase）通过分解细胞壁半纤维素切除半乳糖键而参与果实软化。为了阐明香蕉（Musasp．）果实成熟过程中的软化与细胞壁代谢酶β-半乳糖苷酶基因表达之间的关系,采用RT-PCR方法,从成熟香蕉果实果肉中分离了编码β-半乳糖苷酶基因的部分cDNA（MA-Gal）,序列分析表明,MA-Gal包含927bp,编码309个氨基酸,包含5个β-半乳糖苷酶结构域（典型真核生物中β-半乳糖苷酶包含7个结构域）,推导的MA-Gal蛋白质中有β-半乳糖苷酶蛋白的催化活性部位GGPIILSQIENEY（F）;系统进化树分析结果表明MA-Gal属于第一类β-半乳糖苷酶基因（该类主要在果实中表达）;β-半乳糖苷酶活性和硬度的变化表明其与香蕉果实硬度变化密切相关;Northern分析显示,跃变前期的果肉中,MA-Gal基因的表达量很低,后随着果实的软化表达量不断增加,并在呼吸跃变后达到最高。所有结果表明,MA-Gal参与香蕉果实成熟过程中的软化。     

Distribution and Properties of Endo-β-1,4-glucanase from a Lower Termite,Coptotermes formosanus (Shiraki)

A multi-enzyme distribution of endo-β-1,4-glucanase activity was found in the digestive system of a worker caste of the lower termite Coptotermes formosanus (Shiraki) by zymogram analysis. Its distribution analysis demonstrated that about 80% of this activity was localized in salivary glands from where only one component (EG-E) was secreted into the digestive tract.

EG-E was isolated by a combination of chromatographic and electrophoretic techniques. Its molecular mass, optimal pH and temperature, isoelectric point, and K _m were 48 kDa, 6.0, 50°C, 4.2, and 3.8 (mg/ml on carboxymethylcellulose), respectively. EG-E hydrolyzed cellooligosaccharides with a degree of polymerization of 4 and larger, and had low activity on crystalline cellulose. Main reaction products from low molecular weight cellulose were cellobiose and cellotriose. The N-terminal amino acid sequence of EG-E has similarity with fungal endo-β-1,4-glucanases and cellobiohydrolases of the glycosyl hydrolase family 7 rather than the other insect endo-β-1,4-glucanases of family 9.     

Purification and Characterization of Two Endo-β-1,4-glucanases from Mollusca, Ampullaria crossean

Two novel endo-β-1,4-glucanases, EG45 and EG27, were isolated from the gastric juice of mollusca, Ampullaria crossean, by anion exchange, hydrophobic interaction, gel filtration and a second round of anion exchange chromatography. The purified proteins EG45 and EG27 appeared as a single band on sodium dodecylsulfate polyacrylamide gel electrophoresis with a molecular mass of 45 kDa and 27 kDa, respectively. The optimum pH for CMC activity was 5.5 for EG45 and 4.4-4.8 for EG27. The optimum temperature range for EG27 was broad, between 50℃ and 60 ℃; for EG45 it was 50 ℃. The analysis on the stability of these two endo-β-1,4-glucanases showed that EG27 was acceptably stable at pH 3.0-11.0 even when the incubation time was prolonged to 24 h at 30 ℃, whereas EG45 remained relatively stable at pH 5.0-8.0. About 85% of the activity of EG27 could be retained upon incubation at 60 ℃ for 24 h. However, less than 10% residual activity of EG45 was detected at 50 ℃. Among different kinds of substrates, both enzymes showed a high preference for carboxymethyl cellulose. EG45, in particular, showed a carboxymethyl cellulose hydrolytic activity of 146.5 IU/mg protein. Both enzymes showed low activities to xylan （from oat spelt） and Sigmacell 101, and they were inactive to p-nitrophenyl-β-D-cellobioside, salicin and starch.     

纤维素酶的研究进展

纤维素酶是糖苷水解酶的一种,它可以将纤维素物质水解成简单糖,进而发酵产生乙醇,从而解决农业、再生能源以及环境污染等问题。初期的研究主要集中在对微生物纤维素酶的研究,随着对纤维素酶研究的不断深入,“动物自身不含纤维素酶”这一传统理论被推翻,动物纤维素酶成为纤维素酶研究的热点。另外,生物化学、分子生物学以及基因工程等多种交叉学科的快速发展,获得适合工业化的高比活力的纤维素酶已指日可待。     

肥城佛桃果实软化过程中的超弱发光及其与乙烯释放的关系

无论在室温还是低温条件下,肥城佛桃(Prunus persica cv.Fei-Cheng)果实在衰老软化过程中超弱发光均有明显的高峰出现,其出现时间与乙烯释放速率峰值相一致。乙烯合成抑制剂2-氨基乙氧基乙烯甘氨酸(2-aminoethoxyvinylglycine,AVG)与乙烯利(ethrel,化学名称2-氯乙基膦酸)处理结果显示,果实超弱发光并不随乙烯释放速率的增减而定量变化,说明果实乙烯释放与超弱发光变化没有直接的因果关系,超弱发光高峰的出现可能是果实衰老软化过程中代谢活跃的反映。     

Induction and Impact of Cell Wall Degrading Enzymes in Nutrient Solution of Closed Hydroponic Systems

The potential of the microflora in nutrient solutions to produce cell wall degrading enzymes (CWDE) was investigated by adding glucose or substrates of CWDE, such as chitin, cellulose, curdlan and preparations of fungal mycelia (0, 0.01 and 0.1%, w/v). The results indicate the potential of the microflora in nutrient solutions to produce proteolytic, chitinolytic, cellulolytic as well as β‐1,3‐glucanolytic enzymes. All enzyme complexes were induced by addition of preparations of Fusarium oxysporum f. sp. cyclaminis (Focy) and Pythium ultimum, respectively. In contrast, addition of glucose to nutrient solution resulted in only slight increase of protease and chitinase. No correlation between increased activity of CWDE and survival of Focy was found.