胡椒(Piper nigrum L.)离体培养叶片和芽外植体表面灭菌方案的研究

W. P. D. S. Gunawardhana, P. Perera, H. M. A. P. Muhandiram, D. Swarnathilaka, K. Priyadarshani
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摘要

传统上,花椒是通过茎插枝和种子繁殖的,但由于异花传粉的习惯,种子往往产生具有较高变异的后代。植物组织培养技术是快速克隆繁殖最有效、最可靠的方法,但内生微生物污染限制了组织培养技术的成功。在2种芽型(顶芽和腋芽)和3个不同成熟阶段(第一、第三和第五叶)上试验了12种表面处理方案,以优化培养起始条件。60个外植体采用完全随机设计。使用PC - SAS的Proc CatMod程序对计数数据进行方差的最大似然分析。采用方差分析对连续资料进行分析,采用最小显著差异进行均值分离。结果表明,最佳的灭菌方案是针对外植体类型的。植株顶部的第3片叶片和顶芽是组织污染和褐变最小的最佳外植体。真菌污染多见于叶片外植体,而细菌污染多见于芽外植体。方案含有70%乙醇(30s), 0.1%盐酸(5min),无菌蒸馏水加活性炭(1gl - 1);25 min)和20%次氯酸钠(NaOCl) (15 min)与70%乙醇(1 min)对第三叶的处理效果相当。在顶芽中,0.1%盐酸(10分钟)和70%乙醇(1分钟)的处理方案,以及10% NaOCl(15分钟)和70%乙醇(1分钟)的处理方案具有最高的存活率和最低的污染率。强调了通过控制浓度和暴露时间与70%乙醇结合,以无毒的NaOCl取代有害的hgcl2的潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Surface sterilization protocols of leaf and bud explants for initiating in vitro cultures of Piper nigrum L. (Pepper)
Piper nigrum L. is traditionally propagated by stem cuttings and seeds, but seeds tend to produce progenies with higher variations due to cross - pollination habits. Plant tissue culture technique is the most efficient and reliable method for rapid clonal multiplication, however, endophyte microbial contamination limits the success. Twelve surface protocols were tested on two bud types (apical and axillary buds) and three different maturity stages of the leaf (first, third and fifth leaves) to optimize the conditions for culture initiation. The Completely Randomized Design was used with 60 explants. Maximum likelihood analysis of variance was conducted using the Proc CatMod procedures of PC - SAS to analyse the count data. The continuous data were analysed using Analysis of Variance and the mean separation was done using Least Significant Difference. Results revealed that the optimal sterilization protocol was specific to the explant type. The third leaf from the top of the plant and the apical bud was the best explants giving minimum tissue contamination and browning. Fungal contamination was frequent in leaf explants whereas bacteria in bud explants. The protocols containing 70% ethanol (30s), 0.1% HgCl 2 (5 min) and sterile distilled water with activated charcoal (1 gL - 1 ; 25 min), and 20% sodium hypochlorite (NaOCl) (15 min) with 70% ethanol (1 min) were comparable for the third leaf. In apical buds, the protocols of 0.1% HgCl 2 (10 min) and 70% ethanol (1 min), and 10% NaOCl (15 min) with 70% ethanol (1 min) provided comparable performances with the highest survival and least contamination rates. The potential of replacing hazardous HgCl 2 with non - toxic NaOCl by manipulating the concentration and the exposure time in combination with 70% ethanol was highlighted.
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