Assessment of the genetic fidelity of true-to-type regenerants of medicinal plant Rheum emodi using RAPD and ISSR molecular markers

IF 0.2 Q4 Biochemistry, Genetics and Molecular Biology Research Journal of Biotechnology Pub Date : 2023-08-15 DOI:10.25303/1809rjbt1980204
Sweta Upadhyay, Anjali Uniyal, Vijay Kumar, Sanjay Gupta
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Abstract

Rheum emodi commonly known as rhubarb is mainly found in Northern Himalayas. It is a valuable medicinal plant having major pharmacological activities such as antimicrobial, anticancer, antioxidant, anti-inflammatory and is used extensively as purgative, stomachic and astringent tonic and improves gastro related problems. This herb is used by the local communities for medicinal as well as common eating purpose. This leads to its immense decline in its natural habitat and now this herb falls under threatened species and demands conservation. In this prospective, an efficient in vitro propagation method from callus culture has been achieved using leaf explants excised from the juvenile plant of R. emodi. Murashige and Skoog (MS) basal medium was used for regeneration procedure with different concentration of phytohormones. Maximum frequency of callus formation (84.44±0.27%) was observed in MS+36.19μM (2, 4-D) in combination with 11.10μM (BAP). The highest percentage of adventitious shoot regeneration was observed as 75.56±0.27% and the maximum number of shoots per explant that is 3.67±0.27 was achieved on MS basal medium containing BAP (35.5 μM) and Kn (11.61 μM). The maximum frequency of rooting was observed in MS full strength media + IAA (28.55 μM) + BAP (8.88 μM). The highest frequency of roots per shoot was observed as 5.0±0.47 with an average root length of 11±1.25mm. For ascertaining the clonal fidelity, 20 ISSR markers and 15 RAPD markers were assayed and employed to validate the true-to-type regenerants of Rheum emodi. Out of 15 RAPD and 20 ISSR markers, 7 markers and 15 markers produced distinct, clear and scorable bands with an average of 4.5 bands and 4.4 bands per marker respectively among the tissue cultured progenies. For each primer, the banding pattern was uniform and comparable to mother plant and showed about 99% homology. All the markers produce the monomorphic bands and no variation was detected among the micropropagated plants. Thus, the analysis of ISSR and RAPD patterns revealed that the bands were shared by both in vitro raised plants and parent clump confirming the genetic stability. DNA based molecular markers have proved to be versatile tools in diverse fields of biology. These markers proved to be model tools for routine analysis of clonal fidelity of micropropagated plants prior to commercialization.
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利用RAPD和ISSR分子标记评价药用植物大黄真型再生体的遗传保真度
大黄,俗称大黄,主要分布在喜马拉雅山北部。它是一种珍贵的药用植物,具有抗菌、抗癌、抗氧化、抗炎等重要药理活性,被广泛用于通便、健胃、收敛和改善胃相关问题。这种草药被当地社区用于医药和普通的食用目的。这导致其自然栖息地的急剧减少,现在这种草药属于濒危物种,需要保护。在此基础上,研究了一种有效的愈伤组织离体繁殖方法。采用MS (Murashige and Skoog)培养基,在不同浓度的植物激素条件下进行再生。MS+36.19μM (2,4 - d) + 11.10μM (BAP)的愈伤组织形成频率最高,为84.44±0.27%。在含BAP (35.5 μM)和Kn (11.61 μM)的MS基质上,外植体不定芽再生率最高,为75.56±0.27%,每个外植体不定芽数最高,为3.67±0.27。MS全强培养基+ IAA (28.55 μM) + BAP (8.88 μM)的生根频率最高。平均根长为11±1.25mm,单枝生根频率最高,为5.0±0.47 mm。为了确定大黄的克隆保真度,对20个ISSR标记和15个RAPD标记进行了检测,并对大黄的真型再生物进行了验证。在15个RAPD标记和20个ISSR标记中,7个标记和15个标记在组织培养后代中产生了明显、清晰和可评分的条带,平均每个标记分别为4.5条和4.4条。各引物条带分布均匀,与母株相当,同源性约为99%。所有标记均产生单态条带,在不同的微繁植株间无差异。因此,ISSR和RAPD模式分析表明,这些条带在离体培养植株和亲本丛中都是共享的,证实了遗传稳定性。基于DNA的分子标记已被证明是生物学各个领域的通用工具。这些标记被证明是在商业化之前对微繁殖植物克隆保真度进行常规分析的模型工具。
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来源期刊
Research Journal of Biotechnology
Research Journal of Biotechnology 工程技术-生物工程与应用微生物
CiteScore
0.60
自引率
0.00%
发文量
192
审稿时长
1.5 months
期刊介绍: We invite you to contribute Research Papers / Short Communications / Review Papers: -In any field of Biotechnology, Biochemistry, Microbiology and Industrial Microbiology, Soil Technology, Agriculture Biotechnology. -in any field related to Food Biotechnology, Nutrition Biotechnology, Genetic Engineering and Commercial Biotechnology. -in any field of Biotechnology related to Drugs and Pharmaceutical products for human beings, animals and plants. -in any field related to Environmental Biotechnolgy, Waste Treatment of Liquids, Soilds and Gases; Sustainability. -in inter-realted field of Chemical Sciences, Biological Sciences, Environmental Sciences and Life Sciences. -in any field related to Biotechnological Engineering, Industrial Biotechnology and Instrumentation. -in any field related to Nano-technology. -in any field related to Plant Biotechnology.
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