• 생태와환경
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• 제46권2호
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• pp.276-288
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• 2013

본 연구는 질소 시비에 의해 증가된 토양 질소가 식물의 성장 및 식물체의 화학적 조성에 미치는 영향과 이로 인한 분해에서의 변화를 확인하고자 야외성장실험과 분해실험을 진행하였다. 온실에서 질소 시비구와 비시구 토양에 각각 벼를 재배하였으며 식물이 성숙한 뒤 수확하여 C, N, lignin, cellulose 함량을 측정하였다. 대조구와 질소 처리구 토양에서 재배된 식물의 개체 당 평균 건중량은 각각 0.70 g, 1.32 g로 질소 시비에 의해 1.9배 증가하였다. 식물체의 N 및 C 함량은 질소 시비에 의해 증가하였고 lignin, C/N, lignin/N, cellulose/N은 감소하였다. 이후, 수확된 식물의 지상부는 microcosm 분해실험에 이용되었으며, 분해 식물체에서 건중량의 변화, microbial biomass C와 microbial biomass N, 그리고 dehydrogenase와 urease 활성을 측정하고, 분해과정 중 발생하는 $CO_2$의 양을 정량하였다. 대조구 토양에서 분해시킨 대조구 식물체와 질소 처리구 식물체, 그리고 질소를 처리한 토양에서 분해시킨 질소 처리구 식물체의 잔존량은 각각 초기 건중량의 53.0%, 47.1%, 53.6%를 나타내었다. 질소 시비는 식물체에서 N 함량을 높이고 C/N 및 lignin/N을 낮추어 식물체의 분해를 촉진하였으나, 분해 과정에서의 토양 질소처리는 분해를 억제하였다. 질소 시비에 의해 토양에서 microbial biomass C와 dehydrogenase 활성은 감소하였고, 반면에 microbial biomass N과 urease 활성은 증가하였다. 분해 중 발생한 $CO_2$의 양은 30일 이후부터 질소 시비에 의해 감소하였다. 분해 식물체에서 측정된 microbial biomass C는 질소 처리에 의해 초기에 증가하였으나 이후 저해되는 양상을 나타냈으며 microbial biomass N은 유의한 차이를 보이지 않았다. 질소 시비에 의해 분해 식물체에서 dehydrogenase 활성은 저해되었으며 urease는 분해 초기에 가장 높은 활성을 보였으나 분해 후기에 현저한 감소를 나타냈다. 본 실험에서 질소 시비는 식물의 성장을 증가시키고 식물체의 N 함량을 높여 화학적 조성의 변화를 일으키며 분해율을 증가시키나 분해 단계에서 질소의 시비는 미생물의 활성을 억제시켜 분해를 저해하는 결과를 나타내었다.

• 한국자원식물학회:학술대회논문집
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• 한국자원식물학회 2003년도 춘계 학술발표대회
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• pp.61-62
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• 2003

Clonal propagation of high-value forest trees through somatic embryogenesis (SE) has the potential to rapidly capture the benefits of breeding or genetic engineering programs and to improve raw material uniformity and quality. A major barrier to the commercialization of this technology is the low quality of the resulting embryos. Several factors limit commercialization of SE for Corsican pine, including low initiation rates, low culture survival, culture decline causing low or no embryo production, and inability of somatic embryos to fully mature, resulting in low germination and reduced vigour of somatic seedlings. The objective was to develop a Corsican pine maturation medium that would produce cotyledonary embryos capable of germination. Treatments were arranged in a completely randomized design. Data were analyzed by analysis of variance, and significant differences between treatments determined by multiple range test at P=0.05. Corsican pine (Pinus nigra var. maritima) cultures were initiated on modified !P6 medium. Modifications of the same media were used for culture multiplication and maintenance. Embryogenic cultures were maintained on the same medium semi solidified with 2.5 g/l Gelrite. A maturation medium, capable of promoting the development of Corsican pine somatic embryos that can germinate, is a combination of iP6 modified salts, 2% maltose, 13% polyethylene glycol (PEG), 5 mg!l abscisic acid (ABA), and 2.5 g/l Gelrite. After initiation and once enough tissue developed they were grown in liquid medium. Embryogenic cell suspensions were established by adding 0.951.05 g of 10- to 14-day-old semisolid-grown embryogenic tissue to 9 ml of liquid maintenance media in a 250ml Erlenmeyer flask. Cultures were then incubated in the dark at 2022$^{\circ}$C and rotated at 120 rpm. After 2.53 months on maturation medium, somatic embryos were selected that exhibited normal embryo shape. Ten embryos were placed horizontally on 20 ml of either germination medium ($\frac{2}{1}$strength Murashige and Skoog (1962) salts with 2.5 g/l activated charcoal) or same medium with copper sulphate adjusted to 0.25 mg/1 to compensate for copper adsorption by activated carbon. 2% and 4% maltose was substituted by 7.5% and 13% PEG respectively to improve the yield of the embryos. Substitution of' maltose with PEG was clearly beneficial to embryo development. When 2% of the maltose was replaced with 7.5% PEG, many embryos developed to large bullet-shaped embryos. At latter stages of development most embryos callused and stopped development. A few short, barrel-shaped cotyledonary embryos formed that were covered by callus on the sides and base. When 4% of the maltose was removed and substituted with 13% PEG, the embryos developed further, emerging from the callus and increasing yield slightly. Microscopic examination of the cultures showed differing morphologies, varying from mostly single cells or clumps to well-formed somatic embryos that resembled early zygotic embryos only liquid cultures with organized early-stag. A procedure for converting and acclimating germinants to growth in soil and greenhouse conditions is also tested. Seedling conversion and growth were highly related to the quality of the germinant at the time of planting. Germinants with larger shoots, longer, straighter hypocotyls and longer roots performed best. When mature zygotic embryos germinate the root emerges, before or coincident with the shoot. In contrast, somatic embryos germinate in reverse sequence, with the cotyledons greening first, then shoot emergence and then, much later, if at all, the appearance of the root. Somatic seedlings, produced from the maturation medium, showed 100% survival when planted in a field setting. Somatic seedlings showed normal yearly growth relative to standard seedlings from natural seed.