Storage, manipulation and delivery of DNA fragments is crucial for synthetic biology applications, subsequently allowing organisms of interest to be engineered with genes or pathways to produce desirable phenotypes such as disease or drought resistance in plants, or for synthesis of a specific chemical product. However, DNA with high G+C content can be unstable in many host organisms including
Saccharomyces cerevisiae
. Here, we report the development of
Sinorhizobium meliloti
, a nitrogen-fixing plant symbioticα-Proteobacterium, as a novel host that can store DNA, and mobilize DNA to
E
.
coli
,
S
.
cerevisiae
, and the eukaryotic microalgae
Phaeodactylum tricornutum
. To achieve this, we deleted the
hsdR
restriction-system in multiple reduced genome strains of
S
.
meliloti
that enable DNA transformation with up to 1.4 x 10
5
and 2.1 x 10
3
CFU μg
-1
of DNA efficiency using electroporation and a newly developed polyethylene glycol transformation method, respectively. Multi-host and multi-functional shuttle vectors (MHS) were constructed and stably propagated in
S
.
meliloti
,
E
.
coli
,
S
.
cerevisiae
, and
P
.
tricornutum
. We also developed protocols and demonstrated direct transfer of these MHS vectors via conjugation from
S
.
meliloti
to
E
.
coli
,
S
.
cerevisiae
, and
P
.
tricornutum
. The development of
S
.
meliloti
as a new host for inter-kingdom DNA transfer will be invaluable for synthetic biology research and applications, including the installation and study of genes and biosynthetic pathways into organisms of interest in industry and agriculture.
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