Agrobacterium Mediated Transformation Optimizations for Sugarcane (Saccharum Officinarum L.) Cultivar SPF-234 with Direct Organogenesis

M. Nawaz, N. Iqbal, Rabia Hameed, Mehwish Mehwish, S. Jamil
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Abstract

Sugarcane (Saccharum officinarum L.) is the most important food and energy crop worldwide. In the present study, an efficient Agrobacterium mediated transformation and regeneration system for sugarcane cultivar SPF-234 was established. Agrobacterium tumefaciens strains EHA101and LBA4404 using vector pIG121 Hm, having GUS, HPTII and NPTII genes were used. Polymerase chain reaction (PCR) and histochemical assays confirmed the GUS gene expression. A 620 bp fragment from GUS positive plants was amplified. The GUS expressing putative transformants were 35% of the total plants formed under 30 minute immersion time and 72 hr of incubation period. The co-cultivation media having 60 μM acetosyringone produced 66% GUS expressing plants for LBA4404 and 58% for EHA101. The maximum average number of directly produced shoot (59.5%) from leaf explant was in M6 media having 1.00 mg/l 6-Benzylaminopurine (BAP) and 2.5 mg/l Naphthaleneacetic acid (NAA). A significant decrease (17%) was observed when auxin (NAA) concentration was increased to 4.0 mg/l. The best response of shoot elongation was observed in SE4 media having equal concentration (2.00 mg/l) of both kinetin and BAP. Increased concentrations of kinetin significantly decreased shoot elongation of the subject cultivar. Agrobacterium strain LBA4404 performed better for genetic transformation of the said sugarcane cultivar.This quick and less expensive transformation and direct regeneration system could be exploited for sugarcane on commercial scale in general, and for this elite cultivar in particular.
农杆菌介导的甘蔗转化优化直接器官发生的品种SPF-234
甘蔗(Saccharum officinarum L.)是全球最重要的粮食和能源作物。本研究建立了一种高效的农杆菌介导的甘蔗品种SPF-234转化再生体系。采用载体为pIG121 Hm的农杆菌eha101和LBA4404菌株,分别具有GUS、HPTII和NPTII基因。聚合酶链反应(PCR)和组织化学检测证实GUS基因表达。从GUS阳性植株中扩增出620 bp的片段。在浸泡时间为30分钟、孵育时间为72小时的条件下,表达推定转化体的GUS占植株总数的35%。在含有60 μM乙酰丁香酮的共培养培养基中,LBA4404和EHA101分别有66%和58%的GUS表达植株。在6-苄基氨基嘌呤(BAP)浓度为1.00 mg/l、萘乙酸(NAA)浓度为2.5 mg/l的M6培养基上,叶片外植体直接产芽数最高(59.5%);当生长素(NAA)浓度增加到4.0 mg/l时,细胞凋亡率显著降低(17%)。动素和BAP浓度相等(2.00 mg/l)的SE4培养基对芽伸长的响应最好。动素浓度的增加显著降低了主体品种的茎伸长。农杆菌LBA4404对该甘蔗品种的遗传转化效果较好。这种快速、廉价的转化和直接再生系统一般可用于商业规模的甘蔗,特别是该优良品种。
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