Table 1.

Transformation in Prunus persica L.

Genotype	Method (Strain)	Plasmid (Genes)	Explant	T.E. a (%)	Main Advantage	Main Disadvantage	Reference
“14DR60”	A. tumefaciens (A281)	pGA472 (nptII)	Embryogenic callus, leaves, and immature embryos	0	All three starting explants developed calli, which were able to grow in a medium containing the selective agents.	Typically, long-term embryogenic peach cultures produce few normal shoots.	Scorza et al. [15]
“Tennessee natural”
“PER 2D”
“Redhaven”	A. tumefaciens (tms328::Tn5)	pTiA6 (iaa, ipt)	Shoots	0	Demonstration of potential for using A. tumefaciens to transfer genes to peach.	Shoots could not be regenerated from the transformed cells.	Hammerschlag et al. [16]
			Immature embryo axes	n.s.	Demonstration of regeneration of plants from embryo-derived callus infected with the shooty mutant strain of A. tumefaciens.	Not reproduced in other laboratories.	Smigocki and Hammerschlag [5]
“Lovell”	Biolistic	pBI505, pBI426 (nptII, gus)	Embryo calli, immature embryos, cotyledons, leaves, and shoot tips	0	Optimization of biolistic parameters for this species.	Unsuccessful recovery of plants from the transformed embryogenic calli.	Ye et al. [17]
“Miraflores”	A. tumefaciens (C58C1/pMP90)	pBin19-sgfp (nptII, gfp)	Mature embryo axes	3.6	Mature seeds are available year-round.	Not reproduced in other laboratories.	Pérez-Clemente et al. [12]
“Bailey”	A. tumefaciens (LBA4404, EHA105, GV3101, CG937, CG1052, CG1059)	pLC101 (nptII, gfp)	Cotyledons, embryonic axis, hypocotyl slices, callus, internodes, and leaves	0	Comprehensive evaluation of factors affecting A. tumefaciens-mediated peach transformation. Seed-derived internodes showed the highest transformation percentage compared to the other explants.	Rates of GFP transformation under the experimental conditions were low.	Padilla et al. [18]
“Lady Nancy”
“Harrow Beauty”
“KV930465”	A. tumefaciens (LBA4404, EHA105)	pBin19 (nptII, gus)
“KV930408”
“KV930303”
“KV939455”	A. tumefaciens (LBA4404)	pBISNI, pGA482Ggi (nptII, gus)
“KV930478”
“KV930311”
“Akatsuki”	Electroporation	pBI221, pE2113-GUS, PL-GUS (gus)	Protoplasts from immature fruits mesocarp	0	The system can be applied for expression analysis of genes isolated from other Rosaceae species.	The period suitable for protoplast isolation is limited to about 1 week.	Honda and Moriguchi [19]
“O’Henry”	A. tumefaciens (GV3101, EHA105)	pBIN-m-gfp5-ER (nptII, gfp)	Immature cotyledons	0.6	Very efficient regeneration protocol.	Explants available for only a limited time each year (50 to 70 days post-bloom). Not reproduced in other laboratories.	Prieto [13]
“Rich Lady”
“GF677” b	A. tumefaciens (GV2206)	hp-pBin19 (nptII)	Meristematic bulks	0.3	The first successful report of a peach rootstock genetic transformation using adult tissue as starting material.	The efficiency of the procedure was relatively poor.	Sabbadini et al. [14]
“Hansen 536” b	A. tumefaciens (EHA105)	pK7WG2-ihp35S-PPV194::eGFP (nptII, gfp, PPV polyprotein hairpin)	Meristematic bulks	0	Uses adult tissues as source of explants.	Shoot regeneration from transgenic calli was not obtained.	Sabbadini et al. [20]
	A. tumefaciens (EHA105, LBA4404, GV3101)	pBISN1 (nptII, gus)	Leaves	0	Adult tissue available year-round.	Only transient transformation was recorded.	Zong et al. [21]
“Shantao”	A. rhizogenes (MSU440)	pMV2G + Ri Plasmid (DsRED1) + (rol genes)	Leaves, hypocotyls, and shoots	27.8 c	This protocol provides a way to evaluate gene functions, genetic engineering, and root-rhizosphere microorganism interaction in peach.	Only transgenic hairy roots were regenerated. Transgenic shoots were not produced.	Xu et al. [22]
“Shengli”				50.9 c
“Lvhuajiuhao”				30.7 c
“Shengli”		pSAK277 (PpMYB10.1)	Shoots	n.s. c

^a Transformation efficiency (number of transgenic shoots obtained per 100 explants). When not indicated, it was not specified (n.s.) by authors. ^b Prunus persica x Prunus amygdalus hybrids. ^c Efficiency of regeneration of transgenic hairy roots.