1. IntroductionAlfalfa (Medicago sativa L.) is a perennial crop with a tetraploid genome [1] {Robins JG, 2007 #73} . Due to the high protein content that is suitable for animals, alfalfa is largely used for livestock feed. The capability of the nitrogen fixation of rhizobial bacterium associated with alfalfa is important for improvement of agriculture nitrogen balance [2] . Being of a perennial nature that covers agriculture fields all seasons, alfalfa plants play important roles in soil conservation and soil ecology [3] [4] . In addition, due to its high biomass and non-human food nature, alfalfa is an attractive crop for producing recombinant proteins and other biomaterials from plants via molecular farming approaches [5] [6] [7] [8] . Like many other crops, genetic engineering is an important approach for alfalfa trait modification and improvement. Development of highly efficient genetic transformation methods for different varieties is important for alfalfa genetic engineering. Alfalfa was a pioneering plant species from which somatic embryogenesis was developed [9] [10] [11] . Alfalfa was also a first crop in which genetic transformation was developed. For the past years, alfalfa biotechnology research has been steadily progressing and numerous papers have been published to report different aspects of alfalfa biotechnology development. This paper reviews the recent research progress in alfalfa genetic engineering, focusing on method development for genetic transformation and application of transgenic research. The paper reviews the topics that are not discussed in recent review papers [12] [13] .
2. Genetic Transformation―Tissue Culture Based Technology2.1. Alfalfa GenotypeEstablishment of a plant in vitro regeneration system is the prerequisite for development of genetic transformation, as almost all crops including alfalfa, at this time, rely on tissue culture systems for transgenic development. Alfalfa regeneration is mainly based on somatic embryogenesis and few studies have reported regeneration of alfalfa via organogenesis. Research has indicated that alfalfa somatic embryogenesis is strongly genotype dependent compared to some other plants, and alfalfa in vitro regeneration has been reported only in very limited genotypes [14] [15] [16] [17] [18] . Given that not all the embryogenic genotypes are transformable, at this time, alfalfa transformation is limited to a few cultivars only [19] - [26] . Accordingly, lack of transformation in many alfalfa cultivars is largely due to the lack of in vitro regeneration system in these genotypes, rather than transformability of these genotypes. In this regard, development and improvement of regeneration technologies, specifically, development of somatic embryogenesis technology, is important for future research to achieve genetic transformation for a large number of alfalfa cultivars and genotypes.
2.2. Explant TypeCompared to many other plant species in which transformation is usually conducted using a single and specific explant, alfalfa genetic transformation can be achieved using different types of explants, such as roots, leaves, stems, petioles and somatic embryos, if the genotypes are feasible for somatic embryogenesis [24] - [34] . Specifically, if a genotype is identified to be embryogenic and regenerable, there is a good chance that somatic embryos can be induced in different types of explants. Accordingly, transformation can be conducted using different types of explants. Tian et al. [35] report genetic transformation using a number of different organs as explants and transgenic plants were recovered from all the explants tested. It appeared that the transformation efficiency was not affected by the explants used, rather it depended on the somatic embryogenesis capacity of the explants.
Study and exploration of alfalfa transformation using different types of explant materials not only provide options to meet different needs and situations, but can also provide possibility for a short time frame and feasibility for transfer of new genes into previously transformed alfalfa plants for multiple trait improvement. Besides using ordinary organs for explant transformation, somatic embryos derived from tissue culture can also be used for transformation in alfalfa. Use of somatic embryos as explants in alfalfa genetic transformation can be conducted via direct and indirect somatic embryogenesis [24] [27] [28] [36] [37] . In direct embryogenesis, somatic embryos were first infected by Agrobacterium. The secondary embryogenesis was induced through direct and spontaneous new embryogenesis from primary somatic embryos without callus phase. This method appeared to be effective for alfalfa transformation. However, molecular analysis, such as Southern blotting, which is essential to confirm transformation, was not conducted in recovered plants [27] [28] [37] . The concern is that selection through direct embryogenesis may be less effective and may result in escapes [27] . In addition, spontaneous embryogenesis appeared to be very genotype specific and thus the technique may be restricted to unique clones and genotypes. Liu et al. [24] report a transformation system which also used somatic embryos as explants. The system was based on cell dedifferentiation or cell reprogramming of somatic embryos induced by plant growth regulators, subsequent induction and development of embryogenic calli, and somatic embryo formation from the calli cultured on plant growth regulator-free medium. The biological and regeneration pathway of secondary embryogenesis reported by Liu et al. [24] is different from direct and repetitive embryogenesis [27] [28] [37] . The transformation reported by Liu [24] could be applied to different genotypes and no escapes were observed. Introduction of multiple genes of interest into previously transformed plants to confer plants with different traits is a direction of wide application of transgenic technology [32] . Use of somatic embryos as explants from transgenic plants to initiate transformation to introduce new genes of interest can reduce the time for development of plants that contain multiple new traits. In addition, the system may be an option for those cultivars in which use of other organs for transformation is difficult.
2.3. Tissue Culture Method and TransformationSince the first report of alfalfa genetic transformation, tissue culture-based method has been the main procedure for alfalfa transformation. Nevertheless, use of other methods has also been attempted. Weeks et al. [38] report an in-planta transformation method in which the seedlings were cut at the apical meristem region and infected by Agrobacterium solution with a combination of a few other procedures. This method avoided using the tissue culture system. In-planta transformation has also been reported in Medicago truncatula which is closely related to alfalfa by taxonomy. In that report, seedlings or flowers were infiltrated with Agrobacterium solution and seeds produced from Agrobacterium-infected plants were harvested and then screened to select transformants [39] . In-planta transformation has a number of advantages over tissue culture-based approach; mainly it can reduce extensive labor work involved in tissue culture and avoid using tissue culture facility which is usually costly. However, few studies have since reported to adapt the in-planta transformation methods described above to alfalfa. This indicates that in-planta transformation is less effective and repeatability is low. At this time, tissue culture is still the main method for alfalfa transformation. Thus, continuous research on improving tissue culture methods is still important for alfalfa transformation development and improvement.
Based on the medium reported by Blaydes [40] and Schenk and Hildebrandt [41] , Tian et al. [29] report development of a method in which embryogenic callus can be maintained for a long period of time without losing the embryogenic capacity and when in need, the callus can be transferred to an embryo development medium for embryo formation and subsequently plant recovery [29] [40] [41] . The advantages of this method concerning transformation is that the callus can be maintained for proliferation for an extended period of time and thus the selection for transgenic calli can be conducted repeatedly on fresh medium. This system can strength the selection to effectively eliminate non-transformed cells and to ensure all the tissues developed and plants recovered are all true transformants [29] . Improvement of tissue culture methods to increase the quality of somatic embryos for effective plant regeneration is an important approach to increase alfalfa transformation. Amini et al. [42] report that the efficiency of alfalfa somatic embryo development was increased to 52% in medium supplemented with natural extract from Cuscuta campestris from 26% when no natural extract was used [42] . Subsequently, alfalfa transformation efficiency was increased from 15.2% to 29.3% using the medium containing natural extract. HPLC and GC/MS analyse of the extract showed that the natural extract contained a high level of ABA and certain compounds that promoted somatic embryo maturation. The study suggests that alfalfa genetic transformation could be limited by inefficient tissue culture system and improvement and optimization tissue culture methods can be an important approach for improvement of transformation efficiency or even for the success of transformation.
2.4. Selection SchemeVarious selectable markers have been used to generate transgenic alfalfa lines [43] . Different types of markers have specific advantages and availability of different selection systems is especially useful for sequential transformation to introduce multiple traits into alfalfa plants [44] [45] . Like many plants, using non-antibiotic and non herbicide-based markers for transformation is very much desired. Furthermore, use of alfalfa plant endogenous genes for selection can avoid use of foreign markers and thus can remove some obstacles for wide application of transgenic technology. Ferradini et al. [34] [46] reported use of an alfalfa endogenous gene to select for alfalfa transformation. Gabaculine is an inhibitor of glutamate 1-semialdehyde and aminotransferase (GSA) is toxic to a many plants [34] [46] . A GSA gene, named MsGSAgr was isolated from alfalfa with point-mutation for gabaculine resistance and was proved to be an efficient selectable marker for alfalfa transformation [34] . Forty three percent of the explants produced somatic embryos with this new selection strategy. This selectable marker gene has also been used in distantly related species including tobacco and wheat for transformation. Because the GSA gene is present in all plants, the authors suggest this endogenous plant gene may be used with similar point-mutation for transformation selection of a wide range of plant species [34] [47] .
Besides markers, an important aspect of successful selection is the promoters that drive the expression of the marker genes in different tissues. This is especially true in alfalfa as transformation in alfalfa can be conducted using different types of explants. CaMV35 promoter has been widely used in plant transformation, even for a marker derived from alfalfa [34] . However, the 35S promoter is virus-derived and commercial application of transgenic plants containing viral promoters or genes can have safety concerns. Tian et al. [35] used a plant constitutive promoter, tCUP [48] , to drive the marker gene expression for alfalfa transformation. tCUP is a cryptic promoter found in tobacco via promoter trap strategy [35] [48] . This promoter showed constitutive expression in various tissues and different plant species. The study showed that the tCUP can direct the nptII marker expression in various organs in alfalfa and successful recovery of transgenic plants was demonstrated [48] . Use of a plant derived constitutive promoter in combination with a plant-derived selectable markers [34] for producing transgenic plants added an important merit to application of transgenic technology in alfalfa.
2.5. Preservation of Transgenic Material and TransgenePreservation of transgenes and transgenic materials is an important issue for the wide application of transgenic technology after transgenic plants are generated. Transgene in plants is usually stored in seeds, and after seed germination, the gene can then pass to the next generation. Nevertheless, after self-cross, a portion (a quarter) of the seeds of F1 plants will lose the transgene due to the heterologous status of transgene in plant genome [49] [50] . Several rounds of self-crossing and generations are required to obtain homozygous plants and seeds that all contain the transgenes [51] . Transgene expression in different transgenic plants derived from different transgenic events varies dramatically due to various factors, such as copy number and insertion site. Accordingly, only a few transgenic plants can show desirable levels of transgene expression. Furthermore, the amount of seeds developed from a desired transgenic plant is handful. Development of other methods for transgene preservation is desirable.
Liu et al. [25] reported development of a new technology for stable transgene preservation and authentic expression of transgene in alfalfa plants. Somatic embryos were first induced from transgenic plants [25] . Somatic embryos were then treated with abscisic acid (ABA) to induce desiccation tolerance [50] [52] [53] [54] [55] . The embryos that acquired desiccation tolerance were subjected to water loss process. The dried embryos can be stored at room temperature for extended periods of time. After rehydration, the dried embryos showed high percentage of viability and exhibited routine germination. Normal plants were developed and recovered. Plants germinated from dried somatic embryos showed normal transgene expression and the gene expression levels were comparable to that of plants developed from somatic embryos without desiccation process. Because there is no transgene segregation as occurs in true seeds of F1 plants, all the embryos produced contain the transgene. This can dramatically reduce the time and labor to produce transgene homozygous plants via self-crossing. A large number of somatic embryos can also be induced from a single transgenic plant and this overcomes the limitation of only a handful amount of true seeds can be obtained from a plant. In addition, the transgenic and dried somatic embryos containing the new genes and proteins can be easily transported to other areas when needed. Dried somatic embryos or artificial seed technology provide a novel and useful method for transgene preservation. In another study by Vdovitchenko and Kuzovkina [56] , “artificial seeds” were produced from genetically transformed roots of Baikal skullcap (Scutellaria baicalensis Georgi) and common rue (Ruta graveolens L.), which are medicinal plants [56] . Although authors used terminology of “artificial seeds”, the transgenic materials used in artificial seeds were root fragments encapsulated in gel coat. After long-term storage at low temperature, new shoots can be induced from the artificial seeds. The new tissues developed contained high and desired levels of flavone contents. The study also described some other advantages of the technology including preservation of valuable materials, easy long distance transportation, and little microorganism infection. The method of using other parts of transgenic plants, rather than somatic embryos subjected to encapsulation as described by Vdovitchenko and Kuzovkina to preserve transgenes may be extended to alfalfa to avoid somatic embryogenesis process [56] .
3. Application of Transformation TechnologyTransgenic technology has been used for trait improvement or adding of new traits to alfalfa, and numerous studies for different attributes have been reported (see recent review [13] [57] ). Besides traditional agricultural trait improvement, such as biotic and abiotic stress resistance, alfalfa has also been explored for recombinant protein production due to its high biomass production [7] [58] . As a non-human food plant, use of alfalfa transgenic plants for new protein production has less public or ethical concerns. For the past years, many genes have been transferred to alfalfa for new protein expression and production. However, commercial production of recombinant proteins using alfalfa has not been well achieved. This part of the review will discuss this issue and potential approaches to increase expression via tissue culture. In addition, improvement of alfalfa forage yield and quality has been challenging via traditional methods [59] [60] , but has become possible via the transgenic approach and thus will be discussed here.
3.1. Increasing Recombinant Protein Expression via Tissue Culture ApproachNumerous new biomolecules, including proteins, enzymes, pharmaceuticals and industrial materials have been expressed in alfalfa via transgenic technology [13] . Transgenic approach has also been used to induce chemical functional groups and molecular structure changes in alfalfa [61] . However, at this time, molecular farming to express new proteins in alfalfa is still largely carried out in the laboratories and has yet to reach commercial production stage. Various factors limit the use of the technology commercially. Low level of accumulation of new proteins is indeed the most limiting factor, and thus, improvement of technologies and development of new systems that can lead to high levels of new protein expression are needed for practical application of molecular farming in alfalfa. Recombinant proteins in alfalfa plants are usually expressed in high biomass organs, such as leaves and stems. However, vegetative organs and tissues are not natural reservoirs for protein accumulation, especially for high amounts of foreign protein expression, and the new proteins in these types of organs tend to be degraded by plant regulatory enzymes [62] . Seeds are natural organs for protein accumulation and may be used for new protein production. However, the protein concentration and contents in seeds for a plant species are already high and the space is “full”. In addition, seed production of alfalfa needs special pollinators, such as bees. Using bees may not be possible in some areas, which has increased difficulty of seed production.
Plant tissue culture has been recently re-studied and appears to be a potential system for high levels of recombinant protein expression via transgenic technology. Somatic embryos resemble zygotic embryos in many aspects and may accumulate higher levels of proteins as true seed. A study by Winkelmann et al. [63] showed that 74% of the proteins expressed in zygotic embryos were also found in a similar pattern to express in somatic embryos of ornamental plant Cyclamen persicum using proteomic analysis [63] . Liu et al. and Fu et al. reported somatic embryos could be used for higher levels of new protein expression [31] [64] . Three heterologous genes of uid, ctb, and hIL-13 coding for different proteins were independently transferred into alfalfa via genetic transformation. Somatic embryos were subsequently induced via tissue culture from transgenic plants carrying these genes. Expression analyses showed somatic embryos accumulated significantly higher amounts of new proteins compared to vegetative organs, such as leaves, stems and roots [31] [64] . The new proteins expressed in somatic embryos also exhibited biological activities. They proposed that somatic embryos may have extra “compartments and spaces” for large amounts of new proteins accumulation compared to true seeds in which the spaces may have already been filled by various proteins. Large numbers of somatic embryos can be produced using small amounts of tissues, somatic embryo production can also be scaled up many folds via bioreactors and can be standardized and industrialized. Also, the time for somatic embryo production is much faster than true seed development. Moreover, research has shown that somatic embryos can be induced in planta via regulating the express of certain genes [65] [66] . In planta somatic embryogenesis, once fully developed, can avoid tissue culture approach for embryogenesis and can reduce the cost associated with tissue culture. Thus, somatic embryos may be used as a new and efficient system for new protein production in alfalfa plants.
Other plant tissue culture systems have also been recently employed to increase recombinant protein expression. Kaldis et al. expressed ER-targeted human interleukin-10 (IL-10) in tobacco BY-2 cell suspension [67] . They reported the accumulation of hIL-10 obtained in cell suspension culture of transgenic line was the highest compared to any other stablely transgenic plant expression systems. The authors report that BY-2 cells can multiply up to 100 fold in just one week, which provides a possibility for a large-scale recombinant protein production. Somatic embryos and cell suspension culture have been established for many plant species and may be explored as alternative systems for new protein expression. Moreover, using tissue culture can confine transgenic plants without growing plants in fields. Indeed, the approved first therapeutic proteins for administration in medical treatments in humans and animals were produced in plant cell suspensions partially because the proteins were produced in contained environment. Further research to improve and optimize tissue culture can lead to development of a new system of molecular farming via plant system.
3.2. Forage Yield and Quality ImprovementBreeding in the early 20th century released many alfalfa cultivars, notably “Atlantic” in 1940, “Ranger” in 1942 and “Vernal” in 1953 [68] . However, yield comparison of the varieties released in 1990s and 1950s showed no significant improvement in alfalfa breeding [59] . Improving alfalfa forage yield through traditional breeding methods appears to be restricted, in part because biomass production depends on a number of factors such as environment, growing seasons and plant genetics [59] [60] .
Progress via traditional breeding aimed at improving forage quality is also limited. Generally, forage quality improvement involves increasing digestibility by reducing indigestible cell wall components, such as lignin, and enhancing nutrient composition (protein, sugar, starch, cellulose contents, etc.) in new alfalfa cultivars [26] [69] . It may not be possible to simultaneously improve all of those traits through traditional breeding methods. Functional genomics and genetics are tools to identify novel genes and molecular markers (for example, quantitative trait loci) controlling important agronomic traits in crop plants. A number of such candidate genes are now being tested to develop breeding strategies for forage yield and quality improvement in alfalfa [13] [26] [69] [70] [71] [72] [73] . For the past several years, transgenic technology has been rapidly developed to improve yields in cereal crops including rice [74] [75] [76] , wheat [77] , maize [78] , barley [79] , and forage crops including switchgrass [80] . Very recently using transgenic approach for alfalfa yield improvement has also been reported [70] [73] . Aung et al. demonstrated that overexpression of homologous MsmiR156 gene delayed flowering, and enhanced shoot branching and biomass production in transgenic alfalfa [73] . In addition, manipulation of heterologous LjmiR156 (a miR156 precursor from Lotus japonicus) also improved biomass production even though MsmiR156 and LjmiR156 transgenes displayed some unique effects on forage quality in transgenic alfalfa [70] . Apart from forage yield improvement, transgenic technology has also been used to enhance forage quality in alfalfa. Expression of chimeric genes encoding a ruminal stable, sulfur amino acid-rich protein from sunflower seed resulted in a significant increase in sunflower seed albumin in transgenic alfalfa leaves [81] . Lignin is a major structural polymer in plant vascular tissues, and its rigidity inhibits rumen fermentation of cell wall polysaccharides. Gene manipulation strategies have thus been developed to reduce lignin content in alfalfa. Boucher showed that down regulation of the gene encoding Cinnamyl alcohol dehydrogenases (CAD); an enzyme that catalyzes the last step in the biosynthesis of lignin precursors altered lignin composition and improved in situ cell wall degradation in transgenic alfalfa [82] . Moreover, lignin modification by down regulating hydroxycinnamoyl coenzyme A: shikimate hydroxycinnamoyl transferase (HCT) resulted in a significant increase in digestibility and lignocellulose processing ability in transgenic alfalfa [69] [83] . Aung et al. (2015a) demonstrated that high level of MsmiR156 overexpression resulted in a significant decrease in lignin and increase in cellulose contents, even though those significant effects on forage quality were not observed in the transgenic alfalfa expressing low and moderate MsmiR156 levels. Similarly, high level of LjmiR156 expression significantly increased starch, total flavonoid and total phenolic contents in transgenic alfalfa [26] [70] . These results clearly indicate that transgenic technology has a high potential to improve such agronomic traits as forage yield and quality, which are rarely achieved through traditional breeding methods in alfalfa.
4. ConclusionAlfalfa is an important forage crop worldwide. Like many other crops, transgenic technology is an important approach for alfalfa trait improvement. For the past years, many studies have contributed to alfalfa transgenic technology development and advancement as well as to crop trait improvement via transgenic technology. Alfalfa is a first crop in which plant in vitro regeneration and transformation technologies were developed. Indeed, transformation in alfalfa is only available, at this time, for a few genotypes and is yet to be developed for the vast majority of varieties and genotypes. In addition, high throughput transformation methods, which are important for genomics and molecular biology research, have not been developed. As transformation in alfalfa is essentially based on in vitro regeneration, a major barrier in alfalfa transformation is that regeneration has not been developed for these plants. Continuous research in tissue culture is important for alfalfa genetic transformation and biotechnology development, which is a major discussion focus of this review. Further development of transformation methods is important for promoting the application of transgenic technology for crop trait improvement, which is yet to be seen. Genome editing, especially CRISPR-Cas, is a new and powerful technology for crop trait improvement and has been reported for many plant species but has yet to be demonstrated in alfalfa. Genome editing is usually conducted through genetic transformation. Development of a highly efficient transformation technology for different alfalfa varieties and genotypes will provide a platform for application of genome editing in alfalfa for trait and quality improvement and modification in the future.
Cite this paperLiu, W.T., Aung, B., Hannoufa, A., Xing, T. and Tian, L.N. (2018) Recent Progress of Transgenic Technology Development for Alfalfa. American Journal of Plant Sciences, 9, 467-482. https://doi.org/10.4236/ajps.2018.93035