- Email: [email protected]
Biogenesis of Plant MicroRNAs
March 2014
ScienceDirect
Vol. 21 No. 1 84-96
Journal of Northeast Agricultural University (English Edition)
Available online at www.sciencedirect.com
Biogenesis of Plant MicroRNAs Kong Wen-wen, Wang Hong-bo, and Li Jing* College of Life Sciences, Northeast Agricultural University, Harbin 150030, China
Abstract: microRNAs (miRNAs) play important regulatory roles in eukaryotic gene expression, predominantly at the posttranscriptional level. Elaborate and diverse biogenesis pathways have evolved to produce miRNAs. miRNA biogenesis is a multistep process including transcription, precursor slicing, methylation, nuclear export, and RNA-induced silencing complex assembly. In the decade, since the first discovery of plant miRNAs, many enzymes and regulatory proteins involved in miRNA biogenesis in plants have been uncovered and a basic picture of miRNA processing is emerging gradually. In this article, we summarized the current study of plant miRNA biogenesis and discussed the multiple integrated steps and diverse pathways of miRNA processing. Key words: miRNA, biogenesis, Arabidopsis thaliana, pathway CLC number: Q74
Document code: A
Article ID: 1006-8104(2014)-01-0084-13
themselves are generated and regulated.
Introduction
The first miRNA was discovered in C. elegans in
MicroRNAs (miRNAs) are 18-25 nt long, single-
was reported in Arabidopsis in 2002 (Reinhart et al.
stranded, regulatory non-coding RNAs derived
2002). The miRNAs biogenesis pathways in animals
from hairpin-like precursors. These small molecules
and plants are now basically established after more
regulate gene expression through mRNA cleavage,
than twenty and ten years investigation, respectively.
translation repression, and DNA methylation (Llave et
Despite both animal and plant miRNAs perform
al., 2002; Mallory et al., 2008; Brodersen et al., 2008;
important roles during their life cycle, there are many
Wu et al., 2010; Sun, 2012). In plants, miRNAs play
different details in animal and plant miRNA biogenesis
important roles in diverse regulatory pathways and are
procedures. In animals, MIRs are transcribed by poly-
involved in almost all the developmental events such
merase II (POL II) similar to plant MIRs transcription,
as leaf shape, floral transition (Liu et al., 2006; Park
while some MIR genes are transcribed by polymerase
et al., 2002) as well as mediating responses to both
III (POL III) (Bartel, 2004; Chen et al. 2004). Then,
abiotic (drought, temperature, salinity) (Wang et al.,
the transcripts are sliced twice, and the first slicing
2012; Feng et al., 2013; Ni et al., 2013; Sunkar et al.,
in animals is the nuclear cleavage of the pri-miRNA,
2007) and biotic (bacteria, viruses) (Brotman et al.,
which liberates a stem loop intermediate, known as
2012; Fagard et al., 2007) environmental conditions.
the pre-miRNA by the Drosha RNase III endonuclease
To further dissect the miRNA regulation network, it
(Lee et al., 2003). By Ran-GTP and Exportin-5, this
is important to understand how miRNA genes (MIRs)
pre-miRNA is transported to the cytoplasm and sliced
1993 by Lee et al. (1993) and the first plant miRNA
Received 6 May 2013 Supported by the National Natural Science Foundation of China (31070265) Kong Wen-wen (1990-), male, Ph. D, engaged in the research of plant molecular biology. E-mail: [email protected] * Corresponding author. Li jing, professor, supervisor of Ph. D student, engaged in the research of plant molecular biology. E-mail: [email protected] E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
by another RNase III endonuclease Dicer for the
(previously known as At-Negative on TATA-less2
second time and formed the miRNA/miRNA* duplex.
[NOT2] and VIRE2-INTERACTING PROTEIN2,
(Lund et al., 2004; Lee et al., 2003; Bernstein et al.,
respectively), was recently found to promote this trans-
2001). In plants, MIRs are only transcribed by RNA
cription through their interaction with Pol II (Fig. 1).
polymerase II (Pol II) to form stem-loop structured
NOT2s also interact with DCL1 and some other slic-
primary microRNA (pri-miRNA) (Xie et al., 2005).
ing factors and thus are functional in subsequent
The Dicer-like1(DCL1) complex then slices the pri-
processing steps (Wang et al., 2013). The transcripts
miRNA twice similar to in animals, while both of them
are modified by adding a 5' cap and a 3' polyadenylate
occurred in nucleus. The base of the stem is cut off in
tail like other coding genes (Xie et al., 2005; Lee
the first slicing and precursor miRNA (pre-miRNA)
et al., 2004; Jones-Rhoades et al., 2006).
is produced, while the loop is removed in the second
Some MIR genes contain introns, which have to
slicing and a duplex of miRNA/miRNA* is formed
be removed before the formation of the stem-loop
(Reinhart et al., 2002). After the miRNA/miRNA*
structure (Aukerman and Sakai, 2003; Nikovics et al.,
duplex formation, the miRNA strand (guide strand)
2006). STABILIZED1 (STA1), a protein functioning
is selected and incorporated into the ARGONAUTE1
in pre-mRNA processing in Arabidopsis, was identi-
(AGO1) component of the RNA-induced silencing
fied to be responsible for the intron splicing of
complex (RISC), which then mediates the repression
miRNA transcripts (Ben et al., 2013) (Fig. 1). A
of gene expressions (Song et al., 2004). Recently,
dramatic reduction in the number of mature miRNAs
increasing numbers of new proteins involved in plant
and an accumulation of unspliced pri-miRNAs was
miRNA biogenesis are being discovered. Here, we
detected in sta1. In addition, the transcript level of
focused on current advancements in plant miRNA
DCL1 was reduced in sta1, indicating that STA1 is
studies, and the integrated processes and diverse
responsible for splicing the pre-mRNAs of DCL1 (Ben
pathways of plant miRNA biogenesis were discussed
et al., 2013). These results suggested that STA1 was
in details.
involved in miRNA biogenesis directly by functioning in pri-miRNA splicing and indirectly by modulating
Transcription of MIR Genes
the DCL1 transcript level (Ben et al., 2013).
The majority of MIR genes are located in intergenic
cribed RNA will fold back into a stem-loop struc-
loci between protein-coding genes, while others are
tured pri-miRNA. The length of pri-miRNAs can be
found in intragenic loci, in either introns or exons
variable and ranges from hundreds to several kilo-
(Rajagopalan et al., 2006; Cui et al., 2009). MIR genes
bases (Szarzynska et al., 2009). Generally, one pri-
are transcribed by Pol II in plants (Xie et al., 2005)
miRNA produces one mature miRNA, but it has been
(Fig. 1). As the important gene expression regulator,
found that pri-miRNAs containing multiple stem-
MIR genes transcribed are under precision regulated.
loop structures can produce more than one miRNA
Recent study found that introns of plant pri-miRNAs
(Merchan et al., 2009; Zhang et al., 2010; Lacombe
can enhance miRNA biogenesis (Bielewicz et al.
et al., 2008).
Based on its own compliment sequence, the trans-
2013). Otherwise, the transcriptional co-activator mediator, a conserved protein known to promote trans-
Slicing of pri- and pre-miRNA
cription of protein-coding genes, is required to recruit
The pri-miRNA undergoes two slicing steps to cut
Pol II to transcript factor-binding sites in MIR pro-
off the loop and the stem separately. The slicing is
moters to regulate MIRs transcript (Kim et al., 2011)
a complicated process and a series of proteins are
(Fig. 1). A pair of NOT2 proteins, NOT2a and NOT2b
involved. http: //publish.neau.edu.cn
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Fig. 1 Biogenesis of plant miRNAs MIR genes are transcribed by Pol II. Their transcription is promoted by the co-activators mediator and NOT2s. For intron-containing MIR genes, introns are spliced by STA1. DDL stabilizes pri-miRNAs. The slicing of pri- and pre-miRNA is catalyzed by DCL1 and the proper slicing entails the concerted action and physical interaction of a set of proteins including DCL1, HYL1, SE, CPL1, CBC, DDL, SIC, TGH, and NOT2s. MOS2 is not localized in the D-body but can facilitate the recruitment of pri-miRNA to the dicing complex. The sliced miRNA/miRNA* duplex is methylated by HEN1. The methylated miRNA duplex (also presumably pre-miRNA or mature miRNA) is then exported to the cytoplasm, possibly dependent on HST or the nuclear pore. HYL1 itself or together with DCL1 directionally loads the methylated miRNA/miRNA* duplex into AGO1, which is associated with a complex containing the chaperone HSP90 and SQN. The guide strand is then selected and regulates gene expression, while the passenger strand is either degraded or in non-canonical conditions, loaded into another RISC. E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
A few miRNAs like miR822, miR839, and miR869
Proteins Involved in Slicing
are sliced primarily by DCL4, possibly due to the
DCL and DRB family
(Rajagopalan et al., 2006; Ben et al., 2009).
The DCL and double-stranded RNA-binding (DRB)
In Arabidopsis, besides the canonical 21-nt
families are very important in plant miRNA produc-
miRNAs, a minor fraction of 23-25 nt miRNAs are
tion. Several members in each family are involved
generated independently from the same miRNA pre-
in miRNA biogenesis and the relationships of the
cursors by DCL3 for a large number of MIR genes
members within and between families result in the
(Vazquez et al., 2008). In rice, dozens of MIR genes
diversity and complexity of miRNA biogenesis.
producing only 24 nt long miRNAs or both canonical
In animals, the slicing of miRNA is catalyzed
and long miRNAs have been found (Wu et al., 2010;
by Drosha (Bartel, 2004; Lee et al., 2003), while in
Wu et al., 2009; Zhu et al., 2008). These DCL3-
plants, it is performed by a homolog of Drosha, DCL1,
dependent long miRNAs were demonstrated to be
which is a key protein in plant miRNA biogenesis
loaded into the AGO4-containing RISC complex
(Park et al., 2002). Loss of DCL1 function results in
and direct DNA methylation at their loci of origin as
severely defective phenotypes. In Arabidopsis, dcl1 is
well as in trans at their target genes (Wu et al., 2010)
embryo lethal (Golden et al., 2002). DCL1 belongs to
(Fig. 2c). The generation of long miRNAs is usually
a multidomain ribonuclease III (RNase III)-like family
dependent on the spatial or temporal expression of
that contains four members, DCL1, DCL2, DCL3, and
DCL3, implying possible competition among DCL
DCL4 in Arabidopsis (Voinnet, 2009). DCL proteins
proteins for miRNA precursor slicing under certain
contain a DExD/H-box RNA helicase domain, a
conditions (Vazquez et al., 2008).
DUF283 RNA-binding domain, a small RNA-binding
DRB proteins have widespread functions in RNA
PAZ domain, two tandem RNase III domains, and two
metabolism (Eamens et al., 2012). In Arabidopsis, the
tandem dsRNA-binding domains (dsRBD) (Margis
DRB family contains five closely related members,
et al., 2006; Liu et al., 2006). The length of small
DRB1-DRB5, all of which are involved in small RNA
RNAs sliced by DCLs is based on the distance between
biogenesis. DRB1, also called HYL1 (HYPONASTIC
the PAZ and RNase III domains (Macrae et al., 2006),
LEAVES1), facilitates pri-miRNA processing and was
consequently DCL enzymes themselves are mole-
verified to associate with DCL1 both in vitro (Lu and
cular rulers controlling the length of the small RNAs
Fedoroff, 2000) and in vivo (Kurihara et al., 2006)
they produce. DCL1 can produce 18-21 nt long RNAs
(Fig. 1, 2a). In hyl1, both spliced and intron-containing
while DCL2, DCL3, and DCL4 mainly produce 22,
pri-miRNAs are accumulated (Vazquez et al., 2004;
24, and 21 nt products, respectively (Voinnet, 2009;
Han et al., 2004) and DCL1 cleavage sites are mis-
Takanashi et al., 2011).
placed, resulting in a lower level of functional mature
DCL1 is believed to be the slicing enzyme for most
miRNA (Vazquez et al., 2004). Therefore, HYL1
plant miRNAs (Park et al., 2002; Reinhart et al.,
is required for efficient and precise cleavage of pri-
2002) (Figs. 1 and 2a), while the other DCLs were
miRNA. However, there are still some functional
originally characterized as proteins that function in
mature miRNAs in the hyl1 null mutant, suggesting
other small RNA biogenesis pathways (Xie et al.,
that additional factors or alternative DRB proteins
2004; Gasciolli et al., 2005). However, DCL4, pre-
are involved in accurate DCL slicing (Kurihara et al.,
viously identified as an enzyme for biogenesis of
2006; Han et al., 2004; Yang et al., 2010).
trans-acting small-interfering RNAs (ta-siRNAs), was
DRB2 was reported to be involved in the maturation
found to be involved in miRNA processing (Fig. 2d).
of subsets of miRNAs. Therefore, another DRB2-medi-
highly complementary fold-backs in these pri-miRNAs
http: //publish.neau.edu.cn
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ated non-canonical miRNA pathway was proposed
or with an alternate RISC complex containing an un-
(Eamens et al., 2012) (Fig. 2b). In this pathway, the
known AGO protein, DRB3 and DRB5 instead (Fig. 2b).
pri-miRNA transcript is recognized alternatively by a
In the subsequent step, AGO1-catalyzed RISC
DCL1/DRB2 pairing complex and is sliced to form a
mediates mRNA cleavage and the DRB3 and DRB5-
miRNA/miRNA* duplex. The selected miRNA strand
containing RISC causes translational repression of the
is associated either with an AGO1-catalyzed RISC
target mRNA (Eamens et al., 2012).
Fig. 2 Biogenesis pathways of plant miRNAs a, The DCL1- and DRB1-dependent miRNA biogenesis pathway. In this canonical miRNA pathway, the MIR gene is transcribed by Pol II to form a stem-loop structured pri-miRNA. The step-loop structure is recognized by the DCL1/DRB1-containing complex and sliced twice to generate a miRNA/miRNA* duplex. The mature miRNA strand is associated with the AGO1 component of the RISC to regulate target gene expression by mRNA cleavage; b, The DCL1- and DRB2-dependent miRNA biogenesis pathway. In this non-canonical pathway, the pri-miRNA transcript is recognized alternatively by a DCL1/DRB2 pairing complex and sliced to form a miRNA/miRNA* duplex. The mature miRNA is associated either with an AGO1-catalyzed RISC to mediate mRNA cleavage or an alternate RISC complex containing DRB3 and DRB5 to repress translation of target mRNA; c, The DCL3-dependent miRNA biogenesis pathway. In this non-canonical pathway, the pri-miRNA transcript is recognized by a DCL3containing complex and sliced to form a miRNA/miRNA* duplex. The 23-25 nt long mature miRNA is loaded into an AGO4-containing RISC to direct DNA methylation at its loci of origin as well as in trans at its target gene; d, The DCL4-dependent miRNA biogenesis pathway. The pri-miRNA transcript is recognized by a DCL4-containing complex and sliced to form a miRNA/miRNA* duplex. In this non-canonical pathway, both DRB2 and DRB4 are required. The mature miRNA is loaded into an AGO1-containing RISC to guide mRNA cleavage. Images a and b are from Eamens et al. (2012).
DRB4 was previously identified to play an im-
by associating with DCL4 (Hiraguri et al., 2005;
portant role in small interfering RNA biogenesis
Nakazawa et al., 2007) (Fig. 2d). DCL4-dependent
E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
miRNA accumulation is strongly reduced in drb4,
selection of the miRNA duplex (Manavella et al.,
indicating that DRB4 is required in DCL4-dependent
2012).
miRNA biogenesis (Fukudome et al., 2011; Pélissier
DAWDLE (DDL), a nuclear RNA-binding protein,
et al., 2011). Furthermore, northern blot hybridization
was shown to stabilize pri-miRNA in miRNA bio-
showed that accumulation of miR839 was reduced in
synthesis (Yu et al., 2008) (Fig. 1). In Arabidopsis,
drb2 and drb4, indicating that DRB2 is also required
mature miRNA accumulation is greatly reduced in the
for DCL4-mediated miRNA accumulation (Vazquez
ddl mutant. DDL is capable of binding pri-miRNA
et al., 2010) (Fig. 2d).
and interacting with DCL1 in vitro. Therefore, it was suggested that DDL could improve the stability of pri-
Other slicing factors
miRNA either by binding to the end of the stem-loop
Serrate (SE) is a C2H2-zinc finger protein localized in
or by the indirect effect of DCL1 recruitment (Yu et
the nucleus (Laubinger et al., 2008). The phenotypes
al., 2008; Rogers and Chen, 2013). DDL binding is
of se show a lot of similarities to other miRNA-
general to RNAs and not specific to pri-miRNA; thus,
processing enzyme mutants (Lu and Fedoroff, 2000;
it is involved in other RNA metabolism, which might
Prigge and Wagner, 2001; Bezerra et al., 2004; Clarke
explain why the ddl mutant showed more serious
et al., 1999; Bollman et al., 2003). It was revealed
developmental deficiencies than those of the dcl1
that most pri-miRNAs are accumulated while mature
mutants (Yu et al., 2008).
miRNAs are reduced in se, and the decreased levels of
CAP BINDING Complex (CBC) is a heterodimer
mature miRNAs are correlated with increased levels
that contains two subunits, CBP80 and CBP20
of their target gene transcripts (Lobbes et al., 2006).
(Laubinger et al., 2008; Gregory et al., 2008), and
SE enhances the accuracy of pri-miRNA cleavage by
binds to the 5' cap structure of Pol II transcripts. Pri-
DCL1 both in vitro (Dong et al., 2008) and in vivo
miRNA is accumulated while mature miRNA is
(Manavella et al., 2012). Thus, SE is required for
reduced in cbp80 and cbp20, indicating that CBC
proper slicing of pri-miRNA (Fig. 1). SE was found
plays a role in the pri-miRNA slicing process (Gregory
to be able to react with most of the pri-miRNA slicing
et al., 2008) (Fig. 1). CBP20 binds to SE in vivo and
proteins like DCL1 and HYL1 (Lobbes et al., 2006;
in vitro, suggesting that CBC might be required for
Machida et al., 2011), and was therefore suggested to
the formation of a pri-miRNA processing center by
work as a scaffold-like protein capable of binding both
interacting with SE (Wang et al., 2013). Like DDL,
proteins and RNA to guide the positioning of miRNA
CBC does not function only in miRNA biogenesis,
precursors toward the DCL1 catalytic site (Machida
as mRNA intron slicing is also suppressed in cbp80
et al., 2011).
and cbp20, suggesting that CBC is required in intron
C-TERMINAL DOMAIN PHOSPHATASE-
slicing (Laubinger et al., 2008; Gregory et al., 2008;
LIKE1 (CPL1), containing TFIIF-interacting CTD
Kim et al., 2008).
phosphatase1-like phosphatase and dsRBD domains,
NOT2s are required in pri-miRNA slicing in addi-
is a recently identified protein that affects the accuracy
tion to promoting MIR gene transcription by inter-
of miRNA maturation (Fig. 1). Loss of CPL1 function
acting with Pol II. NOT2s associate with some key
results in the accumulation of miRNA target mRNAs
miRNA processing factors, including DCL1, CBC,
and inaccurate miRNAs without changing the total
and SE (Fig. 1). Impairment of NOT2s leads to mislo-
miRNA level. It was discovered that CPL1 is recruited
calization of DCL1, suggesting that NOT2 proteins
by SE to the DCL1 complex and dephosphorylates
facilitate efficient recruitment of DCL1 and other
HYL1. Dephosphorylation of HYL1 was found to be
processing factors in miRNA biogenesis. These results
important for accurate miRNA processing and strand
explain why inactivation of NOT2s decreases the http: //publish.neau.edu.cn
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Journal of Northeast Agricultural University (English Edition)
Vol. 21 No. 1 2014
accumulation of both pri-miRNA and mature miRNA
its role in regulating the DRB4 and DCL4-containing
(Wang et al., 2013).
dicing complex (Wu et al., 2013).
TOUGH (TGH) contains G-patch and SWAP domains (Suppressor-of-White-APricot), which often
Direction of slicing
exist within RNA metabolism-related proteins
In animals, the rules for miRNA excision from the
(Calderon-Villalobos et al., 2005), and was found to
precursor are simple because of the uniform size
be a component of the DCL1 slicing complex (Fig. 1).
and shape of the pri-miRNA. In contrast, the stem-
In tgh, the accumulation of both DCL1- and DCL4-
loops of pri-miRNAs in plants are quite variable in
mediated miRNAs is reduced and the transcript levels
both length and secondary structure. Accordingly,
of their pri-miRNAs are increased (Ren et al., 2012).
the mechanism for miRNA precursor recognition by
TGH binds ssRNA but not dsRNA in vitro, so it
the DCL1 complex is more complicated and less well
possibly functions by binding to the loop or the bulge
understood. Most plant pri-miRNAs are sliced in the
of pri- or pre-miRNAs. Unlike HYL1 and SE, TGH
stem-to-loop direction like in animals (Breakfield
does not affect miRNA precision, as evidenced by the
et al., 2012). Analysis of pre-miR172 processing
low ratio of imprecise miRNAs in tgh.
showed that the initial cut by the DCL1 complex is
Sickle (SIC), a hydroxyproline-rich glycoprotein,
located –15 nt from the base of the stem, while the
was recently discovered to be involved in miRNA
loop is removed in the second slicing (Mateos et al.,
biogenesis (Fig. 1). Immunolocalization revealed that
2010; Song et al., 2010; Werner et al., 2010).
SIC and HYL1 were colocalized in nuclear bodies.
Unlike most plant miRNAs, miR159 and miR319
sic exhibited some common phenotypes of mutants
are sliced in the loop-to-base direction (Bologna et al.,
defective in miRNA biogenesis and accumulated
2013). Both miR159 and miR319 have long transcripts
lower levels of a subset of miRNAs and higher levels
and can fold-back into a long double-stranded
of corresponding pri-miRNAs than the wild type (Zhan
backbone. Evidence from detailed mutagenesis
et al., 2012). It remains unknown how SIC functions
experiments showed that pre-miR159 and pre-miR319
in pri-miRNA processing. SIC has a function in sliced
processing begins with a cleavage near the loop
intron decay (Zhan et al., 2012), suggesting a possible
(Bologna et al., 2009; Naqvi et al., 2012). DCL1 then
common mechanism for the cleavage of pri-miRNA
continues to cut the precursor three more times at
hairpins and the decay of sliced introns.
20-22 nt intervals until the miRNA is finally released
MOS2 encodes a G-patch and KOW domain-
(Bologna et al., 2009; Addo-Quaye et al., 2009).
containing RNA-binding protein and was previously
Interestingly, the long precursors of miR319 and
identified to be essential for innate immunity in
miR159 are highly conserved in plants, indicating that
Arabidopsis (Zhang et al., 2005). MOS2 is required for
this processing mechanism is ancient (Bologna et al.,
efficient processing of pri-miRNA through facilitating
2009).
the recruitment of pri-miRNA by the dicing complex, as evidenced by the greatly reduced association
Methylation of miRNA/miRNA* duplex
between HYL1 and pri-miRNA in mos2. Interestingly,
HUA ENHANCER1 (HEN1) is a protein contain-
MOS2 binds pri-miRNA both in vitro and in vivo, but
ing a dsRNA-binding motif and a C-terminal methyl-
does not interact with HYL1, SE, or DCL1 and is not
transferase domain and therefore is able to bind
localized in the D-body which is nuclear processing
dsRNA and deposit a methyl group on to the 2'-OH of
center discussed in the following (Fig. 1). Furthermore,
the 3'-terminal nucleotide (Yang et al., 2006). HEN1
MOS2 is also involved in the biogenesis of ta-siRNA,
plays an important role in miRNA maturation because
which is dependent on DRB4 and DCL4, indicating
of its ability to stabilize the miRNA/miRNA* duplex
E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
(Chen, 2005; Li et al., 2005; Yu et al., 2005) (Fig. 1).
be selected as miRNA (guide strand) while the other
After being sliced from the pre-miRNA, the miRNA/
strand (passenger strand/miRNA*) undergoes degrada-
miRNA* duplex is methylated by HEN1 and thus is
tion. The determinant for this selection was discover-
protected from degradation. The hen1 mutant shows a
ed by bioinformatic analysis and confirmed by arti-
similar phenotype to dcl1 and the 3'-ends of miRNAs
ficial miRNA experiments (Rajagopalan et al., 2006).
are found to have additional nucleotides, primarily
The majority of Arabidopsis miRNAs are preferen-
uridines instead of methylated ends. It was discovered
tially selected over their miRNA* strands because of
that the uridylation of unmethylated miRNAs in
the asymmetric thermodynamic stability of the miRNA/
hen1 is performed by a DNA polymerase β family
miRNA* duplex terminus, and the strand with a wea-
protein, HEN1 SUPPRESSOR1 (HESO1), and that
ker 5'-terminus is preferentially chosen as the miRNA
the uridylation leads to degradation (Ren et al., 2012;
guide strand (Rajagopalan et al., 2006; Eamens et al.,
Zhao et al., 2012). Furthermore, the methylation of
2009).
miRNA duplexes may also act as an export signal to
In addition, DRB1 (HY1) is required for strand
the cytoplasm (Park et al., 2005).
selection as evidenced by the higher level of miRNA* in hyl1 mutants (Eamens et al., 2009). Consistently,
Transportation and selection of mature miRNA
cpl1 mutants accumulate higher levels of miRNA*,
In mammals, Exportin 5 (Exp5) exports pre-miRNAs
indicating that the dephosphorylation of HYL1 by
to the cytoplasm before the mature miRNA is gene-
CPL1 is also required for proper guide strand selection
rated (Lund et al., 2004). In plants, the corresponding
(Manavella et al., 2012). DRB1 may bind to or
transportation process is still not clear and both the
interact with the more thermodynamically stable
transporter and the transported molecules remain
end of the miRNA duplex, and then DRB1 alone,
unknown. HASTY (HST), a nuclear shuttle protein
or in a heterodimer with DCL1, directionally loads
that is homologous to Exp5, was suggested to function
the miRNA duplex to the critical miRNA machinery
by exporting methylated miRNA/miRNA* duplexes
protein AGO1 (Eamens et al., 2009; Matranga et al.,
or single-stranded miRNA to the cytoplasm (Bollman
2005; Tomari et al., 2004; Baumberger et al., 2005)
et al., 2003; Park et al., 2005) (Fig. 1). Reduced accu-
where the guide strand is selected (Fig. 1).
mulation of many miRNAs in hst mutants indicates a role for HST in miRNA biogenesis. However, the
RISC assembly
similarly reduced levels of these miRNAs in both the
The assembly of RISC involves the loading of the
nucleus and cytoplasm do not seem to support the
miRNA/miRNA* duplex into AGO complex and
hypothesis that HST functions in miRNA export (Park
subsequent removal of the miRNA* strand. HEAT
et al., 2005). Several species of miRNA are exported
SHOCK PROTEIN 90 (HSP90) was found to be
to the cytoplasm by an HST-independent mechanism
involved in the assembly process as a molecular
and it was suggested that mRNA transport proteins are
chaperone that binds to AGO1 and facilitates the
possibly involved in this process (Park et al., 2005).
loading of the dsRNA duplex (Iki et al., 2010) (Fig. 1).
In addition, the nuclear pore complex might play a
HSP90 mediates substrate peptide association in
role in miRNA transportation as evidenced by the
response to ATP binding and releases the substrate
reduced accumulation of some miRNAs in mutants
on ATP hydrolysis by changing its conformation (Iki
of the nuclear pore component TRANSLOCATED
et al., 2010).
PROMOTER REGION (TPR) (Jacob et al., 2007)
SQUINT (SQN), a member of the immunophilin
(Fig. 1). Before mature miRNA is generated, one strand
family, facilitates RISC assembly and is able to form
of the methylated miRNA/miRNA* duplex has to
a complex with HSP90, AGO1, and small RNA http: //publish.neau.edu.cn
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Journal of Northeast Agricultural University (English Edition)
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duplexes (Fig. 1). Expression of SQN can rescue the
Interestingly, recent studies indicate that miRNA* can
phenotype of sqn null alleles, while expression of
be active in gene silencing in Drosophila melanogaster,
a mutated SQN showing reduced interaction with
humans, and plants (Ghildiyal et al., 2010; Manavella
HSP90 was unable to rescue the phenotype, indicat-
et al., 2013; Meng et al., 2011) (Fig. 1). Large-scale
ing that interaction with HSP90 is required for
sequencing research demonstrates that some miRNA*s
proper SQN function (Iki et al., 2010; Earley et al.,
are quite abundant and enriched in AGO1 complexes
2011; Smith et al., 2009). ATP hydrolysis induces
and miRNA* guided mRNA cleavage products
dissociation of HSP90 and SQN from the complex,
are detected (Devers et al., 2011). In Arabidopsis
followed by unwinding and release of the miRNA*.
miR171a* was verified to be abundant and trigger the
Finally, a mature RISC that contains AGO1 and
silencing of SU (VAR) 3-9 HOMOLOG8 by associa-
the guide strand miRNA is formed (Fig. 1). Once
tion with the AGO1 complex possibly under tissue-
the mature RISC is formed, the miRNA can guide
specific control (Manavella et al., 2013). Meng et al.
the RISC to repress the expression of target genes
(2011) predicted all of the potential miRNA* target
(Voinnet, 2009).
pairs in rice and Arabidopsis based on degradome sequencing data. Their results suggested widespread
Subcellular organization of miRNA biogenesis
miRNA*-mediated gene regulation in plants, but little
The subcellular organization of miRNA biogenesis is
is known about the exact mechanism.
not very clear so far. Fang and Spector (2007) showed that DCL1 and HYL1 colocalize in discrete nuclear bodies, which are refered as nuclear dicing bodies
Conclusions
(D-bodies). Since several proteins essential for miRNA
In the decade since the first report of plant miRNAs,
processing and pri-miRNAs are also associated with
considerable advances have been made in our under-
D-bodies, they suggested that D-bodies are the nuclear
standing of the biogenesis of miRNAs in plants and
sites for the dicing reaction of DCL1 and protein-
a general picture of plant miRNA biogenesis has
protein interaction of the respective proteins (Fig. 1).
emerged. However, there are still some hazy parts. The
HEN1 and AGO1 localize both in the nucleus and the
nuclear export of miRNA in plants is not as clear as in
cytoplasm, and in nucleus a large nucleoplasmic signal
their metazoan counterparts, with both the transporter
is observed in additional to a low level localization
and transported molecules remaining unknown; the
to D-bodies (Fang and Spector, 2007). Therefore,
mechanisms of some processing factors are also not
the methylation of miRNA/miRNA* duplexes and
yet clear; the generation of functional miRNA* is
the loading of miRNA can be either in cytoplasm
waiting to be discovered.
or in nucleus, with the possibility in nucleoplasm.
Some key protein family (e.g., DCL and DRB)
The molecules that are transported through the
mem-bers that were originally identified as being
nuclear membrane and the proteins responsible for
involved in other small RNA pathways have been
the transporting are still kept unknown. It is of great
found to take part in miRNA processing and can
interest to further discover the detailed cellular basis of
cooperate or compete with their miRNA-producing
miRNA biogenesis.
relatives. The intertwined relationships among these processing proteins have revealed the diversity and
miRNA*
complexity of miRNA biogenesis in plants.
MiRNA* strand is originally considered to be non-
Considering its complexity and the large number
functional and simply removed and degraded
of participating proteins, understanding the regulation
(Rajagopalan et al., 2006; Eamens et al., 2009).
of miRNA biogenesis, especially for spatially and
E-mail: [email protected]
·93·
Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
temporally specific miRNAs, can be quite challenging. However, deep sequencing (Friedländer et al., 2008)
Bologna N G, Schapire AL, Palatnik J F. 2013. Processing of plant microRNA precursors. Brief Funct Genomics, 12(1): 37-45.
and tiling array (Liu et al., 2008) technologies have
Breakfield N W, Corcoran D L, Petricka J J, et al. 2012. High-resolution
allowed the examination of precursor, mature, and
experimental and computational profiling of tissue-specific known
intermediate miRNA molecules at an unprecedented
and novel miRNAs in Arabidopsis. Genome Res, 22(1): 163-76.
global level and provide unlimited potential for further study of plant miRNA.
Brodersen P, Sakvarelidze-Achard L, Bruun-Rasmussen M, et al. 2008. Widespread translational inhibition by plant miRNAs and siRNAs. Science, 320(5880): 1185-90.
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ScienceDirect
Vol. 21 No. 1 84-96
Journal of Northeast Agricultural University (English Edition)
Available online at www.sciencedirect.com
Biogenesis of Plant MicroRNAs Kong Wen-wen, Wang Hong-bo, and Li Jing* College of Life Sciences, Northeast Agricultural University, Harbin 150030, China
Abstract: microRNAs (miRNAs) play important regulatory roles in eukaryotic gene expression, predominantly at the posttranscriptional level. Elaborate and diverse biogenesis pathways have evolved to produce miRNAs. miRNA biogenesis is a multistep process including transcription, precursor slicing, methylation, nuclear export, and RNA-induced silencing complex assembly. In the decade, since the first discovery of plant miRNAs, many enzymes and regulatory proteins involved in miRNA biogenesis in plants have been uncovered and a basic picture of miRNA processing is emerging gradually. In this article, we summarized the current study of plant miRNA biogenesis and discussed the multiple integrated steps and diverse pathways of miRNA processing. Key words: miRNA, biogenesis, Arabidopsis thaliana, pathway CLC number: Q74
Document code: A
Article ID: 1006-8104(2014)-01-0084-13
themselves are generated and regulated.
Introduction
The first miRNA was discovered in C. elegans in
MicroRNAs (miRNAs) are 18-25 nt long, single-
was reported in Arabidopsis in 2002 (Reinhart et al.
stranded, regulatory non-coding RNAs derived
2002). The miRNAs biogenesis pathways in animals
from hairpin-like precursors. These small molecules
and plants are now basically established after more
regulate gene expression through mRNA cleavage,
than twenty and ten years investigation, respectively.
translation repression, and DNA methylation (Llave et
Despite both animal and plant miRNAs perform
al., 2002; Mallory et al., 2008; Brodersen et al., 2008;
important roles during their life cycle, there are many
Wu et al., 2010; Sun, 2012). In plants, miRNAs play
different details in animal and plant miRNA biogenesis
important roles in diverse regulatory pathways and are
procedures. In animals, MIRs are transcribed by poly-
involved in almost all the developmental events such
merase II (POL II) similar to plant MIRs transcription,
as leaf shape, floral transition (Liu et al., 2006; Park
while some MIR genes are transcribed by polymerase
et al., 2002) as well as mediating responses to both
III (POL III) (Bartel, 2004; Chen et al. 2004). Then,
abiotic (drought, temperature, salinity) (Wang et al.,
the transcripts are sliced twice, and the first slicing
2012; Feng et al., 2013; Ni et al., 2013; Sunkar et al.,
in animals is the nuclear cleavage of the pri-miRNA,
2007) and biotic (bacteria, viruses) (Brotman et al.,
which liberates a stem loop intermediate, known as
2012; Fagard et al., 2007) environmental conditions.
the pre-miRNA by the Drosha RNase III endonuclease
To further dissect the miRNA regulation network, it
(Lee et al., 2003). By Ran-GTP and Exportin-5, this
is important to understand how miRNA genes (MIRs)
pre-miRNA is transported to the cytoplasm and sliced
1993 by Lee et al. (1993) and the first plant miRNA
Received 6 May 2013 Supported by the National Natural Science Foundation of China (31070265) Kong Wen-wen (1990-), male, Ph. D, engaged in the research of plant molecular biology. E-mail: [email protected] * Corresponding author. Li jing, professor, supervisor of Ph. D student, engaged in the research of plant molecular biology. E-mail: [email protected] E-mail: [email protected]
·85·
Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
by another RNase III endonuclease Dicer for the
(previously known as At-Negative on TATA-less2
second time and formed the miRNA/miRNA* duplex.
[NOT2] and VIRE2-INTERACTING PROTEIN2,
(Lund et al., 2004; Lee et al., 2003; Bernstein et al.,
respectively), was recently found to promote this trans-
2001). In plants, MIRs are only transcribed by RNA
cription through their interaction with Pol II (Fig. 1).
polymerase II (Pol II) to form stem-loop structured
NOT2s also interact with DCL1 and some other slic-
primary microRNA (pri-miRNA) (Xie et al., 2005).
ing factors and thus are functional in subsequent
The Dicer-like1(DCL1) complex then slices the pri-
processing steps (Wang et al., 2013). The transcripts
miRNA twice similar to in animals, while both of them
are modified by adding a 5' cap and a 3' polyadenylate
occurred in nucleus. The base of the stem is cut off in
tail like other coding genes (Xie et al., 2005; Lee
the first slicing and precursor miRNA (pre-miRNA)
et al., 2004; Jones-Rhoades et al., 2006).
is produced, while the loop is removed in the second
Some MIR genes contain introns, which have to
slicing and a duplex of miRNA/miRNA* is formed
be removed before the formation of the stem-loop
(Reinhart et al., 2002). After the miRNA/miRNA*
structure (Aukerman and Sakai, 2003; Nikovics et al.,
duplex formation, the miRNA strand (guide strand)
2006). STABILIZED1 (STA1), a protein functioning
is selected and incorporated into the ARGONAUTE1
in pre-mRNA processing in Arabidopsis, was identi-
(AGO1) component of the RNA-induced silencing
fied to be responsible for the intron splicing of
complex (RISC), which then mediates the repression
miRNA transcripts (Ben et al., 2013) (Fig. 1). A
of gene expressions (Song et al., 2004). Recently,
dramatic reduction in the number of mature miRNAs
increasing numbers of new proteins involved in plant
and an accumulation of unspliced pri-miRNAs was
miRNA biogenesis are being discovered. Here, we
detected in sta1. In addition, the transcript level of
focused on current advancements in plant miRNA
DCL1 was reduced in sta1, indicating that STA1 is
studies, and the integrated processes and diverse
responsible for splicing the pre-mRNAs of DCL1 (Ben
pathways of plant miRNA biogenesis were discussed
et al., 2013). These results suggested that STA1 was
in details.
involved in miRNA biogenesis directly by functioning in pri-miRNA splicing and indirectly by modulating
Transcription of MIR Genes
the DCL1 transcript level (Ben et al., 2013).
The majority of MIR genes are located in intergenic
cribed RNA will fold back into a stem-loop struc-
loci between protein-coding genes, while others are
tured pri-miRNA. The length of pri-miRNAs can be
found in intragenic loci, in either introns or exons
variable and ranges from hundreds to several kilo-
(Rajagopalan et al., 2006; Cui et al., 2009). MIR genes
bases (Szarzynska et al., 2009). Generally, one pri-
are transcribed by Pol II in plants (Xie et al., 2005)
miRNA produces one mature miRNA, but it has been
(Fig. 1). As the important gene expression regulator,
found that pri-miRNAs containing multiple stem-
MIR genes transcribed are under precision regulated.
loop structures can produce more than one miRNA
Recent study found that introns of plant pri-miRNAs
(Merchan et al., 2009; Zhang et al., 2010; Lacombe
can enhance miRNA biogenesis (Bielewicz et al.
et al., 2008).
Based on its own compliment sequence, the trans-
2013). Otherwise, the transcriptional co-activator mediator, a conserved protein known to promote trans-
Slicing of pri- and pre-miRNA
cription of protein-coding genes, is required to recruit
The pri-miRNA undergoes two slicing steps to cut
Pol II to transcript factor-binding sites in MIR pro-
off the loop and the stem separately. The slicing is
moters to regulate MIRs transcript (Kim et al., 2011)
a complicated process and a series of proteins are
(Fig. 1). A pair of NOT2 proteins, NOT2a and NOT2b
involved. http: //publish.neau.edu.cn
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Fig. 1 Biogenesis of plant miRNAs MIR genes are transcribed by Pol II. Their transcription is promoted by the co-activators mediator and NOT2s. For intron-containing MIR genes, introns are spliced by STA1. DDL stabilizes pri-miRNAs. The slicing of pri- and pre-miRNA is catalyzed by DCL1 and the proper slicing entails the concerted action and physical interaction of a set of proteins including DCL1, HYL1, SE, CPL1, CBC, DDL, SIC, TGH, and NOT2s. MOS2 is not localized in the D-body but can facilitate the recruitment of pri-miRNA to the dicing complex. The sliced miRNA/miRNA* duplex is methylated by HEN1. The methylated miRNA duplex (also presumably pre-miRNA or mature miRNA) is then exported to the cytoplasm, possibly dependent on HST or the nuclear pore. HYL1 itself or together with DCL1 directionally loads the methylated miRNA/miRNA* duplex into AGO1, which is associated with a complex containing the chaperone HSP90 and SQN. The guide strand is then selected and regulates gene expression, while the passenger strand is either degraded or in non-canonical conditions, loaded into another RISC. E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
A few miRNAs like miR822, miR839, and miR869
Proteins Involved in Slicing
are sliced primarily by DCL4, possibly due to the
DCL and DRB family
(Rajagopalan et al., 2006; Ben et al., 2009).
The DCL and double-stranded RNA-binding (DRB)
In Arabidopsis, besides the canonical 21-nt
families are very important in plant miRNA produc-
miRNAs, a minor fraction of 23-25 nt miRNAs are
tion. Several members in each family are involved
generated independently from the same miRNA pre-
in miRNA biogenesis and the relationships of the
cursors by DCL3 for a large number of MIR genes
members within and between families result in the
(Vazquez et al., 2008). In rice, dozens of MIR genes
diversity and complexity of miRNA biogenesis.
producing only 24 nt long miRNAs or both canonical
In animals, the slicing of miRNA is catalyzed
and long miRNAs have been found (Wu et al., 2010;
by Drosha (Bartel, 2004; Lee et al., 2003), while in
Wu et al., 2009; Zhu et al., 2008). These DCL3-
plants, it is performed by a homolog of Drosha, DCL1,
dependent long miRNAs were demonstrated to be
which is a key protein in plant miRNA biogenesis
loaded into the AGO4-containing RISC complex
(Park et al., 2002). Loss of DCL1 function results in
and direct DNA methylation at their loci of origin as
severely defective phenotypes. In Arabidopsis, dcl1 is
well as in trans at their target genes (Wu et al., 2010)
embryo lethal (Golden et al., 2002). DCL1 belongs to
(Fig. 2c). The generation of long miRNAs is usually
a multidomain ribonuclease III (RNase III)-like family
dependent on the spatial or temporal expression of
that contains four members, DCL1, DCL2, DCL3, and
DCL3, implying possible competition among DCL
DCL4 in Arabidopsis (Voinnet, 2009). DCL proteins
proteins for miRNA precursor slicing under certain
contain a DExD/H-box RNA helicase domain, a
conditions (Vazquez et al., 2008).
DUF283 RNA-binding domain, a small RNA-binding
DRB proteins have widespread functions in RNA
PAZ domain, two tandem RNase III domains, and two
metabolism (Eamens et al., 2012). In Arabidopsis, the
tandem dsRNA-binding domains (dsRBD) (Margis
DRB family contains five closely related members,
et al., 2006; Liu et al., 2006). The length of small
DRB1-DRB5, all of which are involved in small RNA
RNAs sliced by DCLs is based on the distance between
biogenesis. DRB1, also called HYL1 (HYPONASTIC
the PAZ and RNase III domains (Macrae et al., 2006),
LEAVES1), facilitates pri-miRNA processing and was
consequently DCL enzymes themselves are mole-
verified to associate with DCL1 both in vitro (Lu and
cular rulers controlling the length of the small RNAs
Fedoroff, 2000) and in vivo (Kurihara et al., 2006)
they produce. DCL1 can produce 18-21 nt long RNAs
(Fig. 1, 2a). In hyl1, both spliced and intron-containing
while DCL2, DCL3, and DCL4 mainly produce 22,
pri-miRNAs are accumulated (Vazquez et al., 2004;
24, and 21 nt products, respectively (Voinnet, 2009;
Han et al., 2004) and DCL1 cleavage sites are mis-
Takanashi et al., 2011).
placed, resulting in a lower level of functional mature
DCL1 is believed to be the slicing enzyme for most
miRNA (Vazquez et al., 2004). Therefore, HYL1
plant miRNAs (Park et al., 2002; Reinhart et al.,
is required for efficient and precise cleavage of pri-
2002) (Figs. 1 and 2a), while the other DCLs were
miRNA. However, there are still some functional
originally characterized as proteins that function in
mature miRNAs in the hyl1 null mutant, suggesting
other small RNA biogenesis pathways (Xie et al.,
that additional factors or alternative DRB proteins
2004; Gasciolli et al., 2005). However, DCL4, pre-
are involved in accurate DCL slicing (Kurihara et al.,
viously identified as an enzyme for biogenesis of
2006; Han et al., 2004; Yang et al., 2010).
trans-acting small-interfering RNAs (ta-siRNAs), was
DRB2 was reported to be involved in the maturation
found to be involved in miRNA processing (Fig. 2d).
of subsets of miRNAs. Therefore, another DRB2-medi-
highly complementary fold-backs in these pri-miRNAs
http: //publish.neau.edu.cn
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Vol. 21 No. 1 2014
ated non-canonical miRNA pathway was proposed
or with an alternate RISC complex containing an un-
(Eamens et al., 2012) (Fig. 2b). In this pathway, the
known AGO protein, DRB3 and DRB5 instead (Fig. 2b).
pri-miRNA transcript is recognized alternatively by a
In the subsequent step, AGO1-catalyzed RISC
DCL1/DRB2 pairing complex and is sliced to form a
mediates mRNA cleavage and the DRB3 and DRB5-
miRNA/miRNA* duplex. The selected miRNA strand
containing RISC causes translational repression of the
is associated either with an AGO1-catalyzed RISC
target mRNA (Eamens et al., 2012).
Fig. 2 Biogenesis pathways of plant miRNAs a, The DCL1- and DRB1-dependent miRNA biogenesis pathway. In this canonical miRNA pathway, the MIR gene is transcribed by Pol II to form a stem-loop structured pri-miRNA. The step-loop structure is recognized by the DCL1/DRB1-containing complex and sliced twice to generate a miRNA/miRNA* duplex. The mature miRNA strand is associated with the AGO1 component of the RISC to regulate target gene expression by mRNA cleavage; b, The DCL1- and DRB2-dependent miRNA biogenesis pathway. In this non-canonical pathway, the pri-miRNA transcript is recognized alternatively by a DCL1/DRB2 pairing complex and sliced to form a miRNA/miRNA* duplex. The mature miRNA is associated either with an AGO1-catalyzed RISC to mediate mRNA cleavage or an alternate RISC complex containing DRB3 and DRB5 to repress translation of target mRNA; c, The DCL3-dependent miRNA biogenesis pathway. In this non-canonical pathway, the pri-miRNA transcript is recognized by a DCL3containing complex and sliced to form a miRNA/miRNA* duplex. The 23-25 nt long mature miRNA is loaded into an AGO4-containing RISC to direct DNA methylation at its loci of origin as well as in trans at its target gene; d, The DCL4-dependent miRNA biogenesis pathway. The pri-miRNA transcript is recognized by a DCL4-containing complex and sliced to form a miRNA/miRNA* duplex. In this non-canonical pathway, both DRB2 and DRB4 are required. The mature miRNA is loaded into an AGO1-containing RISC to guide mRNA cleavage. Images a and b are from Eamens et al. (2012).
DRB4 was previously identified to play an im-
by associating with DCL4 (Hiraguri et al., 2005;
portant role in small interfering RNA biogenesis
Nakazawa et al., 2007) (Fig. 2d). DCL4-dependent
E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
miRNA accumulation is strongly reduced in drb4,
selection of the miRNA duplex (Manavella et al.,
indicating that DRB4 is required in DCL4-dependent
2012).
miRNA biogenesis (Fukudome et al., 2011; Pélissier
DAWDLE (DDL), a nuclear RNA-binding protein,
et al., 2011). Furthermore, northern blot hybridization
was shown to stabilize pri-miRNA in miRNA bio-
showed that accumulation of miR839 was reduced in
synthesis (Yu et al., 2008) (Fig. 1). In Arabidopsis,
drb2 and drb4, indicating that DRB2 is also required
mature miRNA accumulation is greatly reduced in the
for DCL4-mediated miRNA accumulation (Vazquez
ddl mutant. DDL is capable of binding pri-miRNA
et al., 2010) (Fig. 2d).
and interacting with DCL1 in vitro. Therefore, it was suggested that DDL could improve the stability of pri-
Other slicing factors
miRNA either by binding to the end of the stem-loop
Serrate (SE) is a C2H2-zinc finger protein localized in
or by the indirect effect of DCL1 recruitment (Yu et
the nucleus (Laubinger et al., 2008). The phenotypes
al., 2008; Rogers and Chen, 2013). DDL binding is
of se show a lot of similarities to other miRNA-
general to RNAs and not specific to pri-miRNA; thus,
processing enzyme mutants (Lu and Fedoroff, 2000;
it is involved in other RNA metabolism, which might
Prigge and Wagner, 2001; Bezerra et al., 2004; Clarke
explain why the ddl mutant showed more serious
et al., 1999; Bollman et al., 2003). It was revealed
developmental deficiencies than those of the dcl1
that most pri-miRNAs are accumulated while mature
mutants (Yu et al., 2008).
miRNAs are reduced in se, and the decreased levels of
CAP BINDING Complex (CBC) is a heterodimer
mature miRNAs are correlated with increased levels
that contains two subunits, CBP80 and CBP20
of their target gene transcripts (Lobbes et al., 2006).
(Laubinger et al., 2008; Gregory et al., 2008), and
SE enhances the accuracy of pri-miRNA cleavage by
binds to the 5' cap structure of Pol II transcripts. Pri-
DCL1 both in vitro (Dong et al., 2008) and in vivo
miRNA is accumulated while mature miRNA is
(Manavella et al., 2012). Thus, SE is required for
reduced in cbp80 and cbp20, indicating that CBC
proper slicing of pri-miRNA (Fig. 1). SE was found
plays a role in the pri-miRNA slicing process (Gregory
to be able to react with most of the pri-miRNA slicing
et al., 2008) (Fig. 1). CBP20 binds to SE in vivo and
proteins like DCL1 and HYL1 (Lobbes et al., 2006;
in vitro, suggesting that CBC might be required for
Machida et al., 2011), and was therefore suggested to
the formation of a pri-miRNA processing center by
work as a scaffold-like protein capable of binding both
interacting with SE (Wang et al., 2013). Like DDL,
proteins and RNA to guide the positioning of miRNA
CBC does not function only in miRNA biogenesis,
precursors toward the DCL1 catalytic site (Machida
as mRNA intron slicing is also suppressed in cbp80
et al., 2011).
and cbp20, suggesting that CBC is required in intron
C-TERMINAL DOMAIN PHOSPHATASE-
slicing (Laubinger et al., 2008; Gregory et al., 2008;
LIKE1 (CPL1), containing TFIIF-interacting CTD
Kim et al., 2008).
phosphatase1-like phosphatase and dsRBD domains,
NOT2s are required in pri-miRNA slicing in addi-
is a recently identified protein that affects the accuracy
tion to promoting MIR gene transcription by inter-
of miRNA maturation (Fig. 1). Loss of CPL1 function
acting with Pol II. NOT2s associate with some key
results in the accumulation of miRNA target mRNAs
miRNA processing factors, including DCL1, CBC,
and inaccurate miRNAs without changing the total
and SE (Fig. 1). Impairment of NOT2s leads to mislo-
miRNA level. It was discovered that CPL1 is recruited
calization of DCL1, suggesting that NOT2 proteins
by SE to the DCL1 complex and dephosphorylates
facilitate efficient recruitment of DCL1 and other
HYL1. Dephosphorylation of HYL1 was found to be
processing factors in miRNA biogenesis. These results
important for accurate miRNA processing and strand
explain why inactivation of NOT2s decreases the http: //publish.neau.edu.cn
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Journal of Northeast Agricultural University (English Edition)
Vol. 21 No. 1 2014
accumulation of both pri-miRNA and mature miRNA
its role in regulating the DRB4 and DCL4-containing
(Wang et al., 2013).
dicing complex (Wu et al., 2013).
TOUGH (TGH) contains G-patch and SWAP domains (Suppressor-of-White-APricot), which often
Direction of slicing
exist within RNA metabolism-related proteins
In animals, the rules for miRNA excision from the
(Calderon-Villalobos et al., 2005), and was found to
precursor are simple because of the uniform size
be a component of the DCL1 slicing complex (Fig. 1).
and shape of the pri-miRNA. In contrast, the stem-
In tgh, the accumulation of both DCL1- and DCL4-
loops of pri-miRNAs in plants are quite variable in
mediated miRNAs is reduced and the transcript levels
both length and secondary structure. Accordingly,
of their pri-miRNAs are increased (Ren et al., 2012).
the mechanism for miRNA precursor recognition by
TGH binds ssRNA but not dsRNA in vitro, so it
the DCL1 complex is more complicated and less well
possibly functions by binding to the loop or the bulge
understood. Most plant pri-miRNAs are sliced in the
of pri- or pre-miRNAs. Unlike HYL1 and SE, TGH
stem-to-loop direction like in animals (Breakfield
does not affect miRNA precision, as evidenced by the
et al., 2012). Analysis of pre-miR172 processing
low ratio of imprecise miRNAs in tgh.
showed that the initial cut by the DCL1 complex is
Sickle (SIC), a hydroxyproline-rich glycoprotein,
located –15 nt from the base of the stem, while the
was recently discovered to be involved in miRNA
loop is removed in the second slicing (Mateos et al.,
biogenesis (Fig. 1). Immunolocalization revealed that
2010; Song et al., 2010; Werner et al., 2010).
SIC and HYL1 were colocalized in nuclear bodies.
Unlike most plant miRNAs, miR159 and miR319
sic exhibited some common phenotypes of mutants
are sliced in the loop-to-base direction (Bologna et al.,
defective in miRNA biogenesis and accumulated
2013). Both miR159 and miR319 have long transcripts
lower levels of a subset of miRNAs and higher levels
and can fold-back into a long double-stranded
of corresponding pri-miRNAs than the wild type (Zhan
backbone. Evidence from detailed mutagenesis
et al., 2012). It remains unknown how SIC functions
experiments showed that pre-miR159 and pre-miR319
in pri-miRNA processing. SIC has a function in sliced
processing begins with a cleavage near the loop
intron decay (Zhan et al., 2012), suggesting a possible
(Bologna et al., 2009; Naqvi et al., 2012). DCL1 then
common mechanism for the cleavage of pri-miRNA
continues to cut the precursor three more times at
hairpins and the decay of sliced introns.
20-22 nt intervals until the miRNA is finally released
MOS2 encodes a G-patch and KOW domain-
(Bologna et al., 2009; Addo-Quaye et al., 2009).
containing RNA-binding protein and was previously
Interestingly, the long precursors of miR319 and
identified to be essential for innate immunity in
miR159 are highly conserved in plants, indicating that
Arabidopsis (Zhang et al., 2005). MOS2 is required for
this processing mechanism is ancient (Bologna et al.,
efficient processing of pri-miRNA through facilitating
2009).
the recruitment of pri-miRNA by the dicing complex, as evidenced by the greatly reduced association
Methylation of miRNA/miRNA* duplex
between HYL1 and pri-miRNA in mos2. Interestingly,
HUA ENHANCER1 (HEN1) is a protein contain-
MOS2 binds pri-miRNA both in vitro and in vivo, but
ing a dsRNA-binding motif and a C-terminal methyl-
does not interact with HYL1, SE, or DCL1 and is not
transferase domain and therefore is able to bind
localized in the D-body which is nuclear processing
dsRNA and deposit a methyl group on to the 2'-OH of
center discussed in the following (Fig. 1). Furthermore,
the 3'-terminal nucleotide (Yang et al., 2006). HEN1
MOS2 is also involved in the biogenesis of ta-siRNA,
plays an important role in miRNA maturation because
which is dependent on DRB4 and DCL4, indicating
of its ability to stabilize the miRNA/miRNA* duplex
E-mail: [email protected]
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Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
(Chen, 2005; Li et al., 2005; Yu et al., 2005) (Fig. 1).
be selected as miRNA (guide strand) while the other
After being sliced from the pre-miRNA, the miRNA/
strand (passenger strand/miRNA*) undergoes degrada-
miRNA* duplex is methylated by HEN1 and thus is
tion. The determinant for this selection was discover-
protected from degradation. The hen1 mutant shows a
ed by bioinformatic analysis and confirmed by arti-
similar phenotype to dcl1 and the 3'-ends of miRNAs
ficial miRNA experiments (Rajagopalan et al., 2006).
are found to have additional nucleotides, primarily
The majority of Arabidopsis miRNAs are preferen-
uridines instead of methylated ends. It was discovered
tially selected over their miRNA* strands because of
that the uridylation of unmethylated miRNAs in
the asymmetric thermodynamic stability of the miRNA/
hen1 is performed by a DNA polymerase β family
miRNA* duplex terminus, and the strand with a wea-
protein, HEN1 SUPPRESSOR1 (HESO1), and that
ker 5'-terminus is preferentially chosen as the miRNA
the uridylation leads to degradation (Ren et al., 2012;
guide strand (Rajagopalan et al., 2006; Eamens et al.,
Zhao et al., 2012). Furthermore, the methylation of
2009).
miRNA duplexes may also act as an export signal to
In addition, DRB1 (HY1) is required for strand
the cytoplasm (Park et al., 2005).
selection as evidenced by the higher level of miRNA* in hyl1 mutants (Eamens et al., 2009). Consistently,
Transportation and selection of mature miRNA
cpl1 mutants accumulate higher levels of miRNA*,
In mammals, Exportin 5 (Exp5) exports pre-miRNAs
indicating that the dephosphorylation of HYL1 by
to the cytoplasm before the mature miRNA is gene-
CPL1 is also required for proper guide strand selection
rated (Lund et al., 2004). In plants, the corresponding
(Manavella et al., 2012). DRB1 may bind to or
transportation process is still not clear and both the
interact with the more thermodynamically stable
transporter and the transported molecules remain
end of the miRNA duplex, and then DRB1 alone,
unknown. HASTY (HST), a nuclear shuttle protein
or in a heterodimer with DCL1, directionally loads
that is homologous to Exp5, was suggested to function
the miRNA duplex to the critical miRNA machinery
by exporting methylated miRNA/miRNA* duplexes
protein AGO1 (Eamens et al., 2009; Matranga et al.,
or single-stranded miRNA to the cytoplasm (Bollman
2005; Tomari et al., 2004; Baumberger et al., 2005)
et al., 2003; Park et al., 2005) (Fig. 1). Reduced accu-
where the guide strand is selected (Fig. 1).
mulation of many miRNAs in hst mutants indicates a role for HST in miRNA biogenesis. However, the
RISC assembly
similarly reduced levels of these miRNAs in both the
The assembly of RISC involves the loading of the
nucleus and cytoplasm do not seem to support the
miRNA/miRNA* duplex into AGO complex and
hypothesis that HST functions in miRNA export (Park
subsequent removal of the miRNA* strand. HEAT
et al., 2005). Several species of miRNA are exported
SHOCK PROTEIN 90 (HSP90) was found to be
to the cytoplasm by an HST-independent mechanism
involved in the assembly process as a molecular
and it was suggested that mRNA transport proteins are
chaperone that binds to AGO1 and facilitates the
possibly involved in this process (Park et al., 2005).
loading of the dsRNA duplex (Iki et al., 2010) (Fig. 1).
In addition, the nuclear pore complex might play a
HSP90 mediates substrate peptide association in
role in miRNA transportation as evidenced by the
response to ATP binding and releases the substrate
reduced accumulation of some miRNAs in mutants
on ATP hydrolysis by changing its conformation (Iki
of the nuclear pore component TRANSLOCATED
et al., 2010).
PROMOTER REGION (TPR) (Jacob et al., 2007)
SQUINT (SQN), a member of the immunophilin
(Fig. 1). Before mature miRNA is generated, one strand
family, facilitates RISC assembly and is able to form
of the methylated miRNA/miRNA* duplex has to
a complex with HSP90, AGO1, and small RNA http: //publish.neau.edu.cn
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Journal of Northeast Agricultural University (English Edition)
Vol. 21 No. 1 2014
duplexes (Fig. 1). Expression of SQN can rescue the
Interestingly, recent studies indicate that miRNA* can
phenotype of sqn null alleles, while expression of
be active in gene silencing in Drosophila melanogaster,
a mutated SQN showing reduced interaction with
humans, and plants (Ghildiyal et al., 2010; Manavella
HSP90 was unable to rescue the phenotype, indicat-
et al., 2013; Meng et al., 2011) (Fig. 1). Large-scale
ing that interaction with HSP90 is required for
sequencing research demonstrates that some miRNA*s
proper SQN function (Iki et al., 2010; Earley et al.,
are quite abundant and enriched in AGO1 complexes
2011; Smith et al., 2009). ATP hydrolysis induces
and miRNA* guided mRNA cleavage products
dissociation of HSP90 and SQN from the complex,
are detected (Devers et al., 2011). In Arabidopsis
followed by unwinding and release of the miRNA*.
miR171a* was verified to be abundant and trigger the
Finally, a mature RISC that contains AGO1 and
silencing of SU (VAR) 3-9 HOMOLOG8 by associa-
the guide strand miRNA is formed (Fig. 1). Once
tion with the AGO1 complex possibly under tissue-
the mature RISC is formed, the miRNA can guide
specific control (Manavella et al., 2013). Meng et al.
the RISC to repress the expression of target genes
(2011) predicted all of the potential miRNA* target
(Voinnet, 2009).
pairs in rice and Arabidopsis based on degradome sequencing data. Their results suggested widespread
Subcellular organization of miRNA biogenesis
miRNA*-mediated gene regulation in plants, but little
The subcellular organization of miRNA biogenesis is
is known about the exact mechanism.
not very clear so far. Fang and Spector (2007) showed that DCL1 and HYL1 colocalize in discrete nuclear bodies, which are refered as nuclear dicing bodies
Conclusions
(D-bodies). Since several proteins essential for miRNA
In the decade since the first report of plant miRNAs,
processing and pri-miRNAs are also associated with
considerable advances have been made in our under-
D-bodies, they suggested that D-bodies are the nuclear
standing of the biogenesis of miRNAs in plants and
sites for the dicing reaction of DCL1 and protein-
a general picture of plant miRNA biogenesis has
protein interaction of the respective proteins (Fig. 1).
emerged. However, there are still some hazy parts. The
HEN1 and AGO1 localize both in the nucleus and the
nuclear export of miRNA in plants is not as clear as in
cytoplasm, and in nucleus a large nucleoplasmic signal
their metazoan counterparts, with both the transporter
is observed in additional to a low level localization
and transported molecules remaining unknown; the
to D-bodies (Fang and Spector, 2007). Therefore,
mechanisms of some processing factors are also not
the methylation of miRNA/miRNA* duplexes and
yet clear; the generation of functional miRNA* is
the loading of miRNA can be either in cytoplasm
waiting to be discovered.
or in nucleus, with the possibility in nucleoplasm.
Some key protein family (e.g., DCL and DRB)
The molecules that are transported through the
mem-bers that were originally identified as being
nuclear membrane and the proteins responsible for
involved in other small RNA pathways have been
the transporting are still kept unknown. It is of great
found to take part in miRNA processing and can
interest to further discover the detailed cellular basis of
cooperate or compete with their miRNA-producing
miRNA biogenesis.
relatives. The intertwined relationships among these processing proteins have revealed the diversity and
miRNA*
complexity of miRNA biogenesis in plants.
MiRNA* strand is originally considered to be non-
Considering its complexity and the large number
functional and simply removed and degraded
of participating proteins, understanding the regulation
(Rajagopalan et al., 2006; Eamens et al., 2009).
of miRNA biogenesis, especially for spatially and
E-mail: [email protected]
·93·
Kong Wen-wen et al. Biogenesis of Plant MicroRNAs
temporally specific miRNAs, can be quite challenging. However, deep sequencing (Friedländer et al., 2008)
Bologna N G, Schapire AL, Palatnik J F. 2013. Processing of plant microRNA precursors. Brief Funct Genomics, 12(1): 37-45.
and tiling array (Liu et al., 2008) technologies have
Breakfield N W, Corcoran D L, Petricka J J, et al. 2012. High-resolution
allowed the examination of precursor, mature, and
experimental and computational profiling of tissue-specific known
intermediate miRNA molecules at an unprecedented
and novel miRNAs in Arabidopsis. Genome Res, 22(1): 163-76.
global level and provide unlimited potential for further study of plant miRNA.
Brodersen P, Sakvarelidze-Achard L, Bruun-Rasmussen M, et al. 2008. Widespread translational inhibition by plant miRNAs and siRNAs. Science, 320(5880): 1185-90.
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