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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

Here, we provide the detailed protocol of a one-step transformation method mediated by Agrobacterium tumefaciens to produce composite plants.

Abstract

Producing composite plants with transgenic roots and nontransgenic stems and buds using Agrobacterium rhizogenes-mediated hairy root transformation is a powerful tool to study root-related biology. Hairy root transformation is established in a wide range of dicotyledons and in several monocotyledon species and is almost independent of the genotype. The traditional method of hypocotyl injection with A. rhizogenes to obtain composite plants is inefficient, time-consuming, laborious, and frequently causes the death of tender and tiny hypocotyl plants. A highly efficient, one-step hairy root transformation mediated by A. rhizogenes was established previously, which eliminates the need for transplanting after producing hairy roots. In this study, a partial hypocotyl and primary root were removed, the hypocotyl incision site was coated with A. rhizogenes, and then hypocotyls were planted in sterile vermiculite. After 12 days of cultivation, the hypocotyl incision expanded and new hairy roots were induced. This article provides the detailed protocol of a one-step transformation method mediated by A. rhizogenes, with its effectiveness demonstrated by producing composite plants of wild soybean, Solanum americanum, and pumpkin.

Introduction

Agrobacterium rhizogenes is a gram-negative soil bacterium from the family Rhizobiaceae. A. rhizogenes can infect almost all dicotyledons, a few monocotyledons, and individual gymnosperms through wounds, producing hairy roots in infected plants. The bacterium carries the Ri (root-inducing) plasmid, and the T-DNA of the Ri plasmid carries the opine synthesis gene and rol genes (root locus genes). After the T-DNA of the Ri plasmid enters a plant cell and is integrated into a host chromosome, the expression of the rol genes induces production of hairy roots1. A plant binary expression vector carrying a target gene is transformed into A. rhizogenes, and the transformed A. rhizogenes is used to infect a plant. Transgenic roots can be induced in infected plants, producing composite plants containing transgenic roots and nontransgenic stems and buds. Generally, a composite plant can be obtained within 14-20 days. A. rhizogenes-mediated hairy root transformation is generally not limited by genotype in dicotyledonous plants2. The hairy roots produced by A. rhizogenes-infected plants are characterized by a fast growth rate, stable inheritance, and easy operation. Hairy root transformation mediated by A. rhizogenes is currently widely used to study root-related biology. Furthermore, the transformation of hairy roots can also be used to validate and optimize the target-editing efficiency of the CRISPR/Cas9 system3,4,5 and protein subcellular localization. Therefore, hairy root transformation is an important tool in research on plant gene function, metabolic engineering, and interactions between roots and rhizosphere microorganisms6,7,8.

Composite plants containing transgenic roots obtained through hairy root transformation have been widely produced in dicotyledonous plants, especially in legumes. The traditional method of injecting the hypocotyl with A. rhizogenes has been used to produce composite Lotus corniculatus9, soybeans10, tomato11, sweet potatoes12, and many other plants5,8. The hypocotyl-injection method is inefficient and is likely to cause the death of young or tiny hypocotyl plants. Therefore, the method was improved by cutting off the embryonic roots, coating the seedling incision with A. rhizogenes, and then placing the hypocotyl on sterile culture medium for rooting cultivation13. However, those steps are performed in a sterile environment, and the operation steps are relatively cumbersome. In particular, the resulting composite plants need to be transplanted, which increases the amount of work. In previous work, one-step A. rhizogenes-mediated (ARM) hairy root transformation was established in cucumber, soybean, Lotus japonicus, Medicago truncatula, and tomato2,14,15,16,17. The primary root and partial hypocotyl were removed, the incision site of the remaining hypocotyl was coated with transformed A. rhizogenes, and the seedling was then planted into moist sterile vermiculite. After 12 days of cultivation, hairy roots were produced at the incision site. The one-step ARM method is highly efficient and requires less time to produce hairy roots. Transplanting after forming hairy roots is also not necessary. Because microbial contamination can be avoided without transplantation, the one-step ARM method can be particularly useful when studying interactions between plants and microorganisms, such as symbiotic nitrogen fixation between leguminous plants and Rhizobia, and symbioses between plants and arbuscular mycorrhizal fungi. In this paper, a detailed one-step A. rhizogenes-mediated hairy root transformation protocol is provided with examples of composite plants produced in wild soybean, Solanum americanum, and pumpkin. With the protocol, researchers can smoothly perform the one-step ARM transformation.

Protocol

1. Plant growth conditions and A. rhizogenes culture

  1. Seed sowing
    NOTE: Wild soybean seeds were collected in Yanggu County, Liaocheng, China; seeds of S. americanum and pumpkin local variety Yinsu were purchased from a market.
    1. Collect seeds of wild soybean, S. americanum, and the local variety of pumpkin, sow them in vermiculite at a depth of 1 cm, and thoroughly water them. Plant 20 seeds in 8 cm x 11 cm x 9 cm plastic boxes. Cultivate the plants in a growth chamber at 24 ± 2 °C with a 16 h light/8 h dark cycle at approximately 70% relative humidity.
      NOTE: Coats of wild soybean seeds must be broken before sowing. If the research question focuses on interactions between plants and microorganisms, seeds, vermiculite, plastic boxes, and water must be sterilized before use.
    2. Activation and culture of A. rhizogenes K599
      NOTE: The A. rhizogenes K599 strain had one binary vector pRed13052 carrying a red fluorescent reporter gene DsRed2.
      1. Remove the A. rhizogenes strain K599 from a -80 °C freezer, and activate the bacteria on solid LB medium (with 50 mg/L kanamycin and 50 mg/L streptomycin) at 28 °C for 48 h.
      2. Pick out a single clone of strain K599 and culture it in 1 mL of liquid antibiotic-containing LB medium for 12 h.
      3. Evenly spread 500 µL of the bacterial suspension on solid antibiotic-containing LB medium, followed by incubation at 28 °C for 24 h.

2. One-step A. rhizogenes-mediated hairy root transformation method

  1. Hypocotyl incision
    1. After 7 days (define the sowing of the seeds as day 0), seedling cotyledons have just unfolded (Figure 1A), use a sterilized, sharp scalpel to cut approximately 0.5-1 cm of the hypocotyl (Figure 1B). Discard the primary root and some of the partial hypocotyl.
      NOTE: Use the scalpel with care.
  2. K599 inoculation
    1. Coat the hypocotyl incision with K599 bacteria (Figure 1C).
    2. Plant the seedlings in moist vermiculite (Figure 1D).
    3. Infect 30 plants of each species via A. rhizogenes-mediated hairy root transformation. Water each plant with 5 mL of resuspended K599 bacterial suspension (OD600 = 0.5-0.6) in a quarter strength (0.25x) Gamborg B-5 basic medium (Figure 1E).
    4. Cover the pots with a highly transparent plastic bag (Figure 1F) and place them in a growth chamber.

3. Hairy root production

  1. Grow the plants for ~12 days post inoculation, new hairy roots will be induced and generated at the incision site. After 15 days, the hairy root lengths typically reach 2-5 cm (Figure 2).
  2. To determine whether the hairy roots produced are transgenic, examine the expression of reporter genes dependent on the transformed vector in K599.
    1. Detect the expression of the reporter gene DsRed2 using a chemiluminescence imaging system with green excitation light at 540 nm and emission at 600 nm (Figure 2B, Figure 2D, and Figure 2F).

Results

Highly efficient one-step A. rhizogenes-mediated hairy root transformation
Hairy roots were produced at the hypocotyl incision site 12 days after inoculation with engineered K599. Transgenic hairy roots were determined based on the expression of the reporter gene contained in the binary vector. Transgenic roots transformed with the reporter gene DsRed2 of composite wild soybean, S. americanum, and pumpkin were observed under natural (Figure 2A

Discussion

The one-step A. rhizogenes-mediated hairy root method is a simpler and more efficient method for producing composite plants than the hypocotyl-injection method. The one-step ARM method significantly improves the efficiency of hairy root transformation, shortens the time to produce hairy roots, increases the number of hairy roots, and reduces the amount of work involved. The improved transformation protocol is optimal for studies on symbioses between leguminous plants and rhizobia and between plants and arbu...

Disclosures

The authors have no conflicts of interest to declare.

Acknowledgements

This work was supported by the Research Fund of Liaocheng University (318012028) and the Natural Science Foundation of Shandong Province (ZR2020MC034).

Materials

NameCompanyCatalog NumberComments
kanamycinSangon Biotech (Shanghai) Co., Ltd.A506636
LB mediumSangon Biotech (Shanghai) Co., Ltd.B540113
plastic boxLiaoSu8 cm x 11 cm x 9 cm
pumpkinlocal variety Yinsu
streptomycinSangon Biotech (Shanghai) Co., Ltd.A610494 
Tanon-5200Multi machineTanon Co., Ltd., China5200Multichemiluminescence imaging system
tomatolocal variety Zhongshu4
wild soybeancollected in Yanggu County, Liaocheng, China

References

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  5. Liu, S., et al. AtGCS promoter-driven clustered regularly interspaced short palindromic repeats/Cas9 highly efficiently generates homozygous/biallelic mutations in the transformed roots by Agrobacterium rhizogenes-mediated transformation. Frontiers in Plant Science. 13, 952428 (2022).
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  16. Wang, X., et al. Application of AtMYB75 as a reporter gene in the study of symbiosis between tomato and Funneliformis mosseae. Mycorrhiza. 33 (3), 181-185 (2023).
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Agrobacterium RhizogenesHairy Root TransformationComposite PlantsOne step MethodHypocotyl InjectionDicotyledonsMonocotyledonsGene FunctionMetabolic EngineeringRhizosphere MicroorganismsViral Screen MarkersRoot related BiologyWild SoybeanSolanum AmericanumPumpkin

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