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Previous Article | Next Article 
Molecular and Cellular Biology, February 2000, p. 883-891, Vol. 20, No. 3
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Trypanosoma brucei Guide RNA Poly(U)
Tail Formation Is Stabilized by Cognate mRNA
Michael T.
McManus,1
Brian K.
Adler,2
Victoria W.
Pollard,3 and
Stephen
L.
Hajduk1,*
Department of Biochemistry and Molecular
Genetics1 and Department of Medicine,
School of Medicine,2 University of Alabama at
Birmingham, Birmingham, Alabama 35294, and Department of
Microbiology, School of Medicine, University of Pennsylvania,
Philadelphia, Pennsylvania 19104-61483
Received 10 August 1999/Returned for modification 11 October
1999/Accepted 5 November 1999
 |
ABSTRACT |
Guide RNAs (gRNAs) are small RNAs that provide specificity for
uridine addition and deletion during mRNA editing in trypanosomes. Terminal uridylyl transferase (TUTase) adds uridines to pre-mRNAs during RNA editing and adds a poly(U) tail to the 3' end of gRNAs. The
poly(U) tail may stabilize the association of gRNAs with cognate mRNA
during editing. Both TUTase and gRNAs associate with two ribonucleoprotein complexes, I (19S) and II (35S to 40S). Complex II is
believed to be the fully assembled active editing complex, since it
contains pre-edited mRNA and enzymes thought necessary for editing.
Purification of TUTase from mitochondrial extracts resulted in the
identification of two chromatographically distinct TUTase activities.
Stable single-uridine addition to different substrate RNAs is performed
by the 19S complex, despite the presence of a uridine-specific 3'
exonuclease within this complex. Multiple uridines are added to
substrate RNAs by a 10S particle that may be an unstable subunit of
complex I lacking the uridine-specific 3' exonuclease. Multiple
uridines could be stably added onto gRNAs by complex I when the cognate
mRNA is present. We propose a model in which the purine-rich region of
the cognate mRNA protects the uridine tail from a uridine exonuclease
activity that is present within the complex. To test this model, we
have mutated the purine-rich region of the pre-mRNA to abolish
base-pairing interaction with the poly(U) tail of the gRNA. This RNA
fails to protect the uridine tail of the gRNA from exoribonucleolytic
trimming and is consistent with a role for the purine-rich region of
the mRNA in gRNA maturation.
| |
INTRODUCTION |
During kinetoplastid RNA editing,
uridine residues are posttranscriptionally added to or removed from
mitochondrial pre-mRNAs. Editing occurs at specific sites in the mRNA
to produce mature mRNA coding sequences (for recent reviews, see
references 3, 15, and 26).
Current in vitro evidence for kinetoplastid RNA insertional editing
supports the multistep enzymatic process first proposed by Blum et al.
(4, 7, 9, 11, 16, 25). First, an editing site-specific
endonuclease recognizes and cleaves the pre-mRNA. Second, a terminal
uridylyl transferase (TUTase) adds uridine (U) residues to the 3'
terminus of the 5' cleavage fragment, and then an RNA ligase joins the
cleaved halves of the mRNA together, completing one round of
insertional editing. In kinetoplastid RNA deletional editing, the
pre-mRNA contains U residues that must be removed by a U-specific
exonuclease to form a mature mRNA coding sequence (9). In
this model of RNA editing, both the TUTase and the U-specific
exonuclease operate at the same step to help ensure that the proper
number of U residues are added or deleted.
The editing site-specific endonuclease, TUTase, and RNA ligase
activities have been shown to cosediment in glycerol gradients, suggesting that these activities may be part of high-molecular-weight complexes (1, 8, 16, 18, 20, 22, 25). In Trypanosoma brucei, two complexes are proposed to be involved in RNA editing (20). Complex I is a ribonucleoprotein (RNP) that
sediments at 19S and consists of guide RNA (gRNA), TUTase, RNA
ligase, and an editing site-specific endonuclease. Complex II is also
an RNP but sediments at 35S to 40S and contains pre-mRNA in addition to
gRNA, TUTase, RNA ligase, and an editing site-specific endonuclease. Because complex II contains pre-edited mRNA, it is likely to be the
fully assembled active editing complex.
gRNAs are key molecules in the editing process. The specificity of U
addition and/or deletion is directed by these small transcripts, which
can fully base pair with the edited mRNA. Although there are hundreds
of different gRNA sequences, gRNAs have some conserved features. For
example, the 5' ends of all gRNAs contain a 4- to 14-nucleotide anchor
sequence, which is proposed to initiate the RNA editing reaction by
base pairing with the pre-edited mRNA immediately 3' of the editing
site (5, 25). Also, gRNAs contain an internal 30- to
40-nucleotide sequence that is complementary to the edited mRNA and
provides the information for correct editing of the mRNA
(4). gRNAs undergo posttranscriptional addition of U
residues at the 3' terminus (6). The poly(U) tail length varies between about 5 and 24 U residues and is critical for efficient in vitro editing reactions to occur (16, 25). Although the precise function of the U tail is unknown, it has been proposed to
assist in RNA editing by forming a duplex with the purine-rich regions
of the mRNA commonly found at the pre-edited sites (6). In
this way, the U tail could act as a tether and stabilize the 5'
pre-mRNA fragment after endonuclease cleavage. Recently, RNA-RNA cross-linking studies have shown that the U tail may interact with the
pre-mRNA, preferring the purine-rich sites close to the first few
editing sites (17). This idea is attractive, since this base
pairing would increase the stability of what is initially a weak
interaction between the anchor duplex of the gRNA and the pre-mRNA.
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MATERIALS AND METHODS |
Materials.
Nucleotide triphosphates (NTPs) were purchased
from Sigma, and radioactively labeled nucleotides were from DuPont New
England Nuclear. Homopolymers and full-length gRNAs were synthesized on an Applied Biosystems 392 DNA/RNA synthesizer. Bacterial alkaline phosphatase, T7 polymerase, Escherichia coli poly(A)
polymerase, and T4 polynucleotide kinase were purchased from Bethesda
Research Laboratories.
Isolation of mitochondria and glycerol gradient
sedimentation.
Procyclic T. brucei TREU 667 was grown
at 26°C in Cunningham medium supplemented with 10% heat-inactivated
fetal bovine serum and gentamicin sulfate (25 µg/ml) (10).
Cells were harvested when they reached a density of 1 × 107 to 1.5 × 107 cells/ml. Mitochondria
were isolated as described by Rohrer et al. (21).
Mitochondrial extract was prepared and sedimented on a 10 to 30%
glycerol gradient as described by Pollard et al. (20).
Preparation of RNAs.
RNA primers (50 pmol) without a 5'
phosphate were 5' 32P labeled with T4 polynucleotide kinase
in accordance with manufacturer recommendations. For 3'-end labeling,
RNA primers (50 pmol) were extended by a single nucleotide in a 10-µl
reaction mixture containing 1.74 U of poly(A) polymerase, 60 mM KCl, 20 mM Tris (pH 7.8), 5 mM magnesium chloride, 10 mM manganese acetate, and
66 pmol of [
-32P]NTP. All RNAs were gel purified on
preparative denaturing 8% polyacrylamide sequencing gels. The
sequences of the gRNAs used are in the gRNA sequence database
(27). For gA6-[14] and gA6-[48], the 3'-most terminal U
was not included, unless otherwise designated. A6U2 and Cyb
5' mRNA
sequences were transcribed in vitro as previously described (12,
16).
Enzyme assays.
The standard TUTase assay was performed in an
18-µl reaction mixture which consisted of 6 µl of a partially
purified 19S glycerol gradient fraction or 1 µl of the purified
complex, 50 mM KCl, 20 mM Tris (pH 7.9), 5 mM magnesium chloride, 1 mM
UTP, and 1 pmol of RNA substrate (approximately 50,000 cpm). This
reaction mixture was incubated at room temperature for 90 min. Acid
precipitation assays for TUTase were performed as previously described
(20). U-specific exonuclease assays were performed
essentially the same way as the standard TUTase assay, but UTP was
omitted. Ligase adenylation was performed as previously described
(23).
gRNA U-tailing experiments used 1 pmol of a synthetic gRNA for ATPase
subunit 6 mRNA editing (gA6-[14] with no U tail) with or without 5 pmol of cognate ATPase subunit 6 pre-mRNA (A6U2) (16) or
control cytochrome b pre-mRNA (Cyb5') (12) per
assay. When nucleotides were added, the reaction mixtures contained the designated NTP at 1 mM. RNAs were recovered by ethanol precipitation as
described above. Products were separated on a denaturing 8% polyacrylamide sequencing gel containing 7 M urea and visualized by
autoradiography. Quantitation was performed on an Applied Biosystems Storm phosphorimager.
Purification.
Purifications were performed with 20 liters of
T. brucei (approximately 1.5 × 107
cells/liter). Mitochondrial extract was prepared as described previously (20). Extract was cleared by sedimentation
(12,000 × g, 10 min, 4°C) prior to running on a
heparin-Sepharose column (5-ml packed volume; Pharmacia). The column
was washed with buffer A (20 mM Tris [pH 7.9], 100 mM KCl, 1 mM
EDTA). Fractions were eluted with a salt gradient (100 to 600 mM KCl).
Fractions active for single-U addition and ligase (eluting at
approximately 300 mM KCl) were then pooled and diluted with buffer A to
reduce the salt concentration to below 100 mM KCl. This material was
then loaded onto a Q-Sepharose column (1-ml packed volume; Pharmacia). After washing with 150 mM KCl, 1-ml fractions were collected from a 150 to 600 mM KCl 16-ml gradient. Fractions were assayed, and activities
were found to elute at approximately 200 mM KCl. Active fractions were
pooled (2 ml), and proteins were separated on a 10 to 30% glycerol
gradient as previously described (20) except that MgCl was omitted.
Metabolic labeling and isolation of mitochondria.
Metabolic
pulse-labeling of mitochondrial vesicles was performed as previously
described (13). Metabolically labeled mitochondria were
solubilized with Triton X-100, and radiolabeled complexes were
separated on a glycerol gradient (20). Further separation of
labeled complexes was performed on native 3 to 20% acrylamide gels.
Labeled RNAs from glycerol gradient fractions were isolated by
phenol-chloroform extraction and then analyzed on a denaturing 6%
polyacrylamide-7 M urea gel. Pulse-chase experiments were conducted as
for the metabolic labeling experiments, except that excess unlabeled
UTP (5 mM) was added at the designated time points.
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RESULTS |
TUTase activity sediments with 19S and 35S-to-40S complexes.
In order to examine TUTase activity associated with editing complexes,
mitochondrial lysates were fractionated on linear 10 to 30% glycerol
gradients (20). TUTase activity within each fraction was
assayed by measuring the incorporation of [32P]UTP
into trichloroacetic acid-precipitable RNA (Fig.
1). The major peak of TUTase activity
sedimented at 19S, consistent with its being part of previously defined
editing complex I (19S) (20). A second, smaller peak
consistently sedimented at 35S to 40S, suggesting that TUTase activity
is also present in complex II. Gradient fractions containing particles
larger than 40S had no significant TUTase activity.
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FIG. 1.
TUTase activity sediments with RNP complexes.
Mitochondrial extract was sedimented on a 10 to 30% glycerol gradient
and fractionated into 16 fractions, and TUTase activity was measured by
monitoring the incorporation of [32P]UTP into yeast
total tRNA by using the trichloroacetic acid assay as described in
Materials and Methods. Gradient fractions containing complexes I (19S)
and II (35S to 40S) are indicated.
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gRNA poly(U) tail length in complex I and II RNPs.
The next
experiments examined the posttranscriptional addition of UTP into
endogenous gRNAs associated with complexes I and II. Isolated
mitochondria were incubated in the presence of
[-32P]UTP under conditions that suppress
transcription. Previous work has shown that such conditions produce
radiolabeled editing complexes due to incorporation of
[-32P]UTP into RNAs by TUTase (19, 22). The
identities of various labeled RNAs have previously been shown by
hybridization experiments (13). Mitochondrial mRNAs
incorporate UTP because of RNA editing, while 9S and 12S rRNAs receive
long U tails (2), as do gRNAs (6).
Pulse-labeled mitochondria were detergent solubilized, and editing
complexes were separated by centrifugation on glycerol gradients.
Aliquots from each fraction were run on nondenaturing polyacrylamide
gradient gels, and native RNPs were identified by autoradiography (Fig.
2A). Two major RNA-containing complexes were identified in fractions corresponding to 19S complex I and 35S to
40S complex II. To examine the sizes of the gRNAs in the mitochondrial
RNPs, RNA from each fraction was isolated and resolved on denaturing
gels (Fig. 2B). The average sizes of the gRNAs present in these two
editing complexes differed by 15 nucleotides.
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FIG. 2.
Posttranscriptional labeling of isolated mitochondria.
Isolated mitochondria were pulse-labeled with [32P]UTP
under conditions that arrest transcription but support polyuridylation
of gRNAs. Even numbers at the top of both panels A and B represent
glycerol gradient fractions. (A) Native-gel separation of pulse-labeled
mitochondrial RNPs fractionated on a 10 to 30% glycerol gradient.
Fractions containing complexes I and II are indicated. Protein
molecular size markers are indicated in kilodaltons. (B) Analysis of
labeled gRNAs present in complexes I and II from the
posttranscriptional pulse-labeling experiments on denaturing sequencing
gel. Fractions containing complexes I and II are indicated. nt,
nucleotides. (C) Time course of pulse-chase-labeled complex II gRNAs
shown in panel B. Isolated mitochondria were pulsed with
[32P]UTP for 3 min and then incubated with excess
unlabeled UTP for the times shown (for details, see Materials and
Methods). DNA size standards are indicated in nucleotides.
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Pulse-chase experiments also determined the overall kinetics of UTP
incorporation into gRNAs. For these studies, an excess of unlabeled UTP
was added after a 3-min [-32P]UTP pulse. Mitochondria
were incubated for another 10 or 30 min (Fig. 2C), and then the RNAs
were recovered and analyzed on a denaturing gel. The length of complex
II-associated gRNAs increased by approximately 15 nucleotides between
the 3-min pulse and the 10-min chase time. Longer chase times of up to
30 min did not radically increase the size (Fig. 2C, 30 min). The
length of the complex I-associated gRNAs remained short during the
course of the pulse-chase experiments (Fig. 2C, compare complexes II
and I at 30 min). The size distribution of the radiolabeled gRNAs in
complex I is consistent with primary gRNA transcripts lacking a 3'
poly(U) tail. Larger gRNA transcripts, which likely have posttranscriptionally added poly(U) tails of ~15 to 20 nucleotides, are enriched within editing complex II RNPs. These results suggest that
factors within complex II can influence the formation or stability of
the 3' poly(U) tail on gRNAs.
TUTase reactivity on different RNA substrates.
We have
examined nucleotide addition onto different RNAs by glycerol
gradient-purified complex I TUTase. Complex I-associated TUTase
activity was assayed with 5'- or 3'-end labeled gRNAs and poly(A) RNA
in the presence of various nucleotides. This allowed us to evaluate
both nucleotide specificity and RNA preferences. The ability of TUTase
to add U residues to three full-length gRNAs (gA6-[14], gA6-[48],
and gCyb-[558]) was examined. These gRNAs were 5' end labeled and
reacted with TUTase in the presence of GTP, ATP, CTP, UTP, or UTP plus
AMP-CPP. AMP-CPP is an ATP analogue that contains a nonhydrolyzable
-
phosphate bond and is an inhibitor of RNA ligase
(23). gRNAs gA6-[14] and gA6-[48] were excellent substrates for the addition of a single nucleotide (n+1) but not for U
tail formation (Fig. 3A). Single-U
addition to gCyb[558] was also observed (data not shown). A long
exposure of the gel shown in Fig. 3A revealed a small amount of product
which resulted from the addition of multiple U residues; however, the
major product consisted of gRNAs containing one added U. This result
was consistent among different preparations, and often over 60% of the
gRNA could be converted to the n+1 product. The presence of AMP-CPP did
not affect the formation of this n+1 product, and the addition of 1 mM
ATP to UTP-containing reaction mixtures did not promote any further
gRNA elongation. However, the addition of both UTP and ATP promoted the
self-ligation of the gRNA to form circular RNAs (Fig. 3A, ATP+UTP
lane). Consistent with its being a circular RNA, this product migrated
at different positions on different-percentage polyacrylamide
gels (data not shown). The circularization of T. brucei RNAs, including gRNAs, by RNA ligase has previously been described by other groups (22, 28).
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FIG. 3.
U addition to different RNA substrates using glycerol
gradient-purified complex I. (A) Predominately one stable U is added to
gRNAs. 5'-end-labeled gA6-[14] and gA6-[48] were incubated with the
designated NTP at 1 mM. Arrows point to the single-U addition product,
and circles designate circularization of the gRNA by RNA ligase present
in the extract. A minus sign indicates buffer without enzyme. (B) A
poly(A) RNA is a substrate for both a single U addition and a poly(U)
tail. The nucleotides added are indicated at the bottom. The arrow
points to the single-U addition product, and the bracket shows the 10- to 15-nucleotide poly(U) tail. A minus sign represents buffer without
enzyme. The values on the right are numbers of nucleotides. (C) A
5'-end-labeled gA6-[14] gRNA that already contains a single 3' U is
not a substrate for another U. The plus and minus symbols refer to
with- and without-enzyme conditions, respectively. All products were
analyzed by 8% denaturing PAGE and visualized by autoradiography.
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To further examine the substrate preferences of TUTase, we tested
ribohomopolymers poly(G), poly(A), poly(C), and poly(U) for the ability
to serve as substrates for TUTase addition. Both poly(A) (Fig. 3B) and
poly(U) (data not shown) are substrates for the complex I-associated
TUTase, while neither poly(G) nor poly(C) can serve as an efficient
substrate (data not shown). Poly(A) RNA, radiolabeled at the 5' end, is
also very efficient at receiving a single added U (Fig. 3B, arrow).
However, this RNA was unlike any other RNA we had examined in that it
was a substrate for the addition of a distinct 10- to 15-U tail
product. The addition of 10 to 15 U residues was independent of poly(A) substrate RNA length (data not shown). The poly(A) substrate was only
extended in the presence of UTP (Fig. 3B). Neither UMP nor UDP could
substitute for UTP in the extension of the poly(A) substrate (data not
shown). Longer exposures of the autoradiograph revealed that only a
very small amount of other nucleotides could be added onto either
poly(A) or gRNAs (Fig. 3A and B and data not shown). The presence of
ATP along with UTP in these reaction mixtures slightly skewed the
distribution of the U added and considerably increased the amount of
the poly(A) substrate ligation products migrating by about 40 and 60 nucleotides (Fig. 3B, ATP+UTP lane). Interestingly, these ligation
products depended upon the presence of UTP, as ATP alone produced no
ligated poly(A) RNA (Fig. 3B, ATP lane). These results show that the
TUTase activity associated with the 19S complex is specific for UTP and
does not require ATP. To summarize, both gRNAs and poly(A) are
substrates for a major single-U addition, yet only the poly(A) RNA
produced a significant amount of a 10- to 15-nucleotide poly(U) addition.
A polymerase is said to be distributive when only a single nucleotide
is added per binding event. It is possible that the n+1 addition to the
gRNAs is simply the result of U addition by a distributive enzyme and
that the poly(U) tail addition to the poly(A) RNA is the product of a
different enzyme that is not active on the gRNA. In principle, the
major n+1 product could simply be the consequence of limiting amounts
of a distributive enzyme. To test this, we prepared a gRNA substrate
that already contained a 3' added U. When we tested this gRNA in the
TUTase assay, we found that it was not a substrate for U addition (Fig.
3C, compare A6-[14]3'U to control gA6-[14]). Thus, our initial
interpretation was that the n+1 product was not simply a result of
having limiting amounts of a distributive enzyme present.
We also synthesized 5'-end-labeled gRNAs with poly(U) tails varying in
length from 2 to 20 U residues. When complex I TUTase was added to
these reaction mixtures, we observed rapid exonuclease trimming of the
gRNA to a length corresponding to the native gRNA sequence and n+1
product lengths (data not shown). This result is not altogether
surprising, since a 3' U-specific exoribonuclease activity has been
shown to copurify with a functional 19S editing complex
(22). Thus, competing activities of TUTase and 3' U-specific exoribonuclease are present within the glycerol gradient 19S complex I fractions.
Single-U addition copurifies with RNA ligase.
The
above-described experiments did not address the issue of whether the
n+1 addition and the poly(U) tail are the result of a single enzyme or
multiple enzymes. To address this, we purified the TUTase activities
starting from isolated mitochondria. In this purification, we monitored
RNA ligase activity, since RNA ligase can be radiolabeled with ATP and
is therefore a convenient marker for editing complexes (23).
Heparin-Sepharose chromatography was chosen as our initial step in
TUTase purification, since it bound most of the RNA ligase and TUTase
activities and the majority of mitochondrial proteins did not bind.
However, a significant amount of nuclease activity for gRNAs was
present in the fractionation. The poly(A) substrate was more resistant
to nuclease degradation in these assays than gRNAs. For this reason,
poly(A) RNA and gRNA substrates were sometimes substituted in the
TUTase assays. Monitoring of U addition to the poly(A) RNA also allowed
us to assay for both single-U and poly(U) additions.
When we assayed fractions from the heparin-Sepharose separation, we
found that n+1 addition activity was chromatographically distinct from
the multiple-U addition activity on a poly(A) substrate (Fig.
4A). Fractions that contained major 10- to 15-U addition products (lanes 12 to 14) also contained single-U
addition products. The peak of RNA ligase coincided with the single-U
addition activity and not the 10- to 15-nucleotide U addition activity
(Fig. 4A, ligase). We reasoned that fractions containing both TUTase
and RNA ligase activities would be enriched in editing complexes. Thus,
we pooled fractions 9 to 11 for further purification by Q-Sepharose
chromatography.
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FIG. 4.
Single-U addition activity copurifies with RNA ligase
and exonuclease. (A) RNA ligase and multiple-U addition activities are
chromatographically distinct on heparin-Sepharose. A 1-pmol sample of
5'-labeled poly(A) RNA (designated pA20) was incubated with
1 µl of each fraction in the presence of 1 mM UTP. RNA ligase in each
of the corresponding fractions was adenylated and is shown at the
bottom. (B) Single-U addition activity cofractionates with U
exonuclease (U-exo) activity. Fractions 9 to 11 from the
heparin-Sepharose column (A) were pooled and further purified on
Q-Sepharose. A 1-pmol sample of 3'-labeled A6-[14] was incubated with
1 µl of each fraction in the presence of 1 mM UTP. RNA ligase in each
of the fractions was adenylated and is shown at the bottom. For the
exonuclease assay, 1 pmol of 5'-end-labeled poly(U) RNA (designated
pU25) was incubated with 1 µl of each fraction. For the
TUTase assays, single-U addition is shown by an arrow. S, F, and W,
respectively, indicate starting material, flowthrough, and wash. (C)
Silver staining of proteins present in the glycerol gradient
purification step. Fractions 4 and 5 from the Q-Sepharose column (B)
were pooled, and the complexes were separated on a 10-to-30% glycerol
gradient. Following adenylation, protein was isolated and analyzed by
SDS-10% PAGE. Size markers are shown at the left, and sizes are given
in kilodaltons. Gradient fractions are indicated above. An asterisk
indicates the 57-kDa radioactively labeled ligase. (D) Single-U
addition products coincide with a stable 19S complex. A 1-pmol sample
of 5'-labeled poly(A) RNA was incubated with 1 µl of each glycerol
gradient fraction in the presence of 1 mM UTP. RNAs were recovered and
analyzed by 8% urea-PAGE. Adenylated ligase that corresponds to these
fractions is shown at the bottom.
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On Q-Sepharose, most of the RNA ligase and TUTase activity bound while
the majority of proteins flowed through the column during loading. We
were able to analyze single-U addition to a 5'-end-labeled gA6-[14]
RNA across these fractions (Fig. 4B, top). Again, single-U addition
coincided with the peak of RNA ligase (Fig. 4B, middle, lanes 4 to 6).
We also analyzed the fractions for 3' U-specific exoribonuclease across
these fractions (Fig. 4B, bottom), which has been previously shown to
copurify with an editing complex (22). This activity also
peaked in fractions containing a single-U addition and RNA ligase,
suggesting that these activities can reside within the same complex.
In order to determine whether the TUTase activity purified on the
Q-Sepharose column was associated with a stable editing complex, pooled
fractions (4 and 5) were sedimented on a 10 to 30% glycerol gradient.
Proteins in each glycerol gradient fraction were then analyzed by
sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (Fig.
4C). Most of the protein from the Q-Sepharose pool sedimented in
fraction 14, where free protein and small complexes sediment. Bradford
protein assays revealed that combined fractions 11 and 12 contained
approximately 15% of the starting total protein (Table
1). Only ~60% of the adenylated RNA
ligase present in the glycerol gradient sedimented at 19S, suggesting
that some dissociation of the complexes occurred during purification
(Fig. 4D, bottom, ligase). When TUTase was assayed across this
gradient, we found that U addition activity predominately cosedimented
with the 19S complex (Fig. 4D, top, lanes 11 and 12). Interestingly, the 10- to 15-nucleotide U addition activity that was not previously detected in the Q-Sepharose pool was present in the ~10S fractions that contained free protein (Fig. 4C, lanes 13 and 14).
The results of our purification are outlined in Table 1. The single-U
TUTase activity was purified over 1,000-fold. This represents
significant purification, since the starting mitochondrial extract
represents approximately 10% of the total T. brucei
protein. Likewise, ligase was purified over 900-fold, further
supporting the idea that these two enzymes are associated within a
single complex.
In a separate purification scheme, we pursued isolation of the 10- to
15-nucleotide U addition activity. This TUTase activity sedimented at
~10S and contained very little, if any, RNA ligase and 3' U-specific
exonuclease (data not shown). Furthermore, preliminary evidence
suggests that this ~10S particle is a subunit of the 19S complex and
can be dissociated by treatment with a high salt concentration.
Role of mRNA in formation of the gRNA poly(U) tail.
Given that
the 19S complex adds only a single U to gRNAs, we wanted to understand
how the 35S-to-40S complex was able to generate gRNAs containing
poly(U) tails. A major difference between editing complexes I and II is
the presence of pre-mRNA (20). To determine whether the
formation of the gRNA poly(U) tail might be influenced by the presence
of its cognate mRNA, we added synthetic pre-mRNAs to in vitro reaction
mixtures containing purified editing complex and 5'-labeled gRNAs (Fig.
5). The addition of A6U2 pre-mRNA to the
TUTase reactions containing the A6-[14] gRNA resulted in the addition
of approximately 30 to 40 U residues to the gRNA [Fig. 5, lane 5, bracket labeled poly(U) tail]. A shorter exposure of this
autoradiogram revealed a prominent n+1 product (arrow) that was present
in reaction mixtures with and without added mRNA (Fig. 5B, lanes 2, 3, 5, and 6). The addition of noncognate pre-mRNA (Cyb) did not promote
gRNA elongation (lane 6). As expected, a major product present in
reaction mixtures that contained ATP was circular gRNA (Fig. 5A and B,
bracket and circle). Cognate mRNA, but not noncognate mRNA, was
sufficient to abolish gRNA circularization (compare lane 5 to lane 6).
Addition of ATP (compared to UTP alone) to these reaction mixtures
increased the amount, but not the size distribution, of tailed products
(data not shown). These results were also reproduced by using
gCyb[558] and 5'Cyb mRNA substrates (data not shown). The reason
for the ATP stimulation of the poly(U) extension reaction is unclear
but may be ATP-dependent conformational changes in the editing complex.
This possibility remains untested. The ATP stimulation of gRNA
circularization is not unexpected. At low RNA concentrations,
intramolecular ligation and circularization are favored over
intermolecular ligation and dimer formation. Also favoring
circularization is the close proximity of the 5' and 3' ends of gRNAs
(24). For these reasons, it is likely that these gRNAs would
be excellent substrates for self-ligation and form circular RNAs.
Whether circular gRNAs have any physiological relevance or whether they
are simply in vitro artifacts is unknown. Circularization of the gRNAs
could certainly interfere with poly(U) tail formation, since the 3' OH
would be unavailable for poly(U) addition.
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FIG. 5.
Addition of cognate mRNA promotes addition of a stable
poly(U) tail to gRNA. (A) Samples (200 nmol) of synthetic gRNAs with
(+) or without ( ) 1 pmol of cognate mRNA per assay (A6U2). Cognate
mRNA or 1 pmol of nonspecific control RNA (Cyb5' mRNA) was added
with the gRNA prior to the addition of buffer, nucleotides, and
extract. The contents of each reaction mixture are indicated above the
respective lane. The starting substrate gRNA A6-[14] is labeled at
the left, and gRNA gA6-[14] with a poly(U) tail is shown by the
bracket at the right [poly(U) tail]. (B) Lower exposure of the
autoradiogram in panel A. The circle and bracket depict circular gRNA
products, and the arrow depicts single-U addition. Products of the
reactions were resolved by denaturing 8% PAGE and visualized by
autoradiography.
|
|
The efficiency of these reactions is comparable to that of the in vitro
editing reactions (16, 25), with only a small percentage
being converted to poly(U)-tailed gRNA. Phosphorimager analysis
quantitated a 2.5-fold increase in poly(U)-tailed gRNA in reaction
mixtures that contained cognate pre-edited mRNA compared to control
reaction mixtures that contained noncognate pre-mRNA. There was no
significant increase in poly(U) tailing between the reaction mixtures
with no added mRNA and control reaction mixtures with added noncognate
pre-mRNA.
Polypurine-rich region of the pre-mRNA stabilizes the gRNA poly(U)
tail.
In our initial studies with crude editing complexes, we
found that poly(A) ribohomopolymer is a substrate for the addition of
multiple U residues (Fig. 3B). One possible mechanism by which the
poly(A) substrate can receive a strong 10- to 15-nucleotide U tail is
by snap-back hybridization between the newly synthesized poly(U) tail
and the poly(A) substrate sequence. In this model, approximately 10 to
15 U residues would be added by the TUTase, which would then fold back
to hybridize with the poly(A) sequence. The added U residues would be
base paired with the poly(A) substrate and thus be inaccessible to both
TUTase and 3' U-specific exonuclease. In a similar manner, the gRNA
poly(U) tail might interact with purine residues in the pre-mRNA and
thus protect newly added U residues on the gRNA from U-specific
exoribonucleolytic trimming. To test this idea, we created a mutant RNA
(RY) in which the purine-rich region of the pre-edited site was
modified so that it contained predominately pyrimidine residues. This
mutation should abolish base-pairing interactions between the gRNA
poly(U) tail and the mRNA.
In the absence of cognate wild-type mRNA, the poly(U) tail of the gRNA
was trimmed back to the native gRNA sequence by the U-specific
exonuclease present in purified 19S complex (Fig.
6A, no-mRNA lanes). Within 1 min, the
gRNA poly(U) tail was completely cleaved back to the native gRNA
sequence (Fig. 6A, gA6-[14] no U-tail). Addition of cognate wild-type
sequence A6U2 mRNA essentially prevented trimming, and most of the
poly(U) tail remained intact even at the later time points (Fig. 6A,
+WT A6U2 lanes). However, the purine-to-pyrimidine substitution mutant
pre-mRNA could not reproduce this protection (Fig. 6A, +RY lanes),
and at the 5-min time point, most of the U tail was effectively
removed. Thus, the presence of a polypurine region upstream of the
editing site protects the poly(U) tail from degradation, possibly by
A · U and G · U base pairing. The pre-edited region of
the A6U2 mRNA contains a purine-rich region approximately 35 nucleotides long, and can base pair with the poly(U) tail, making the
3' nucleotide inaccessible to exoribonucleolytic trimming. The mutant
RY pre-mRNA, having no purine-rich region to base pair with the
poly(U) tail, is not able to protect from U-specific 3' trimming (Fig.
6B).
View larger version (23K):
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FIG. 6.
Polypurine-rich region of the pre-edited mRNA stabilizes
the gRNA poly(U) tail. (A) The starting RNA substrate is gA6-[14]
with a 17-nucleotide poly(U) tail (gA6-[14]pU17). The
substrate RNA and 19S complex from the Q-Sepharose pool was incubated
in the absence of mRNA (no mRNA), in the presence of cognate wild-type
A6U2 mRNA (+WT A6U2), or in the presence of cognate purine-rich region
substitution mutant mRNA (+RY A6U2). Products of U-specific 3'
exoribonucleolytic trimming are indicated at the left (gA6-[14] no
U-tail). Incubation times are given above the lanes. The arrow labeled
uridine tail trimming indicates the direction of product formation. (B)
Cartoon depicting reactions shown in panel A. In the absence of cognate
wild-type mRNA, the gRNA poly(U) tail is subject to U-specific 3'
exoribonucleolytic trimming. In the presence of cognate wild-type mRNA,
the poly(U) tail can hybridize to the polypurine-rich region on the
mRNA and thus hinder U trimming. In the polypyrimidine-rich mutant, the
U tail cannot base pair with the mRNA and thus is susceptible to U
trimming.
|
|
| |
DISCUSSION |
The results presented here provide several new insights into the
TUTase activity present in T. brucei mitochondria. We found that the 19S editing complex stably added a single U to RNAs. This is
likely due to competing activities between the complex-associated U-specific 3' exonuclease and TUTase. However, gRNAs received multiple
U residues in the presence of cognate mRNA, suggesting that complex II
contains a pool of gRNAs with stable poly(U) tails. We also show that
the polypurine-rich regions within the pre-edited mRNA confer stability
on the gRNA poly(U) tail.
Glycerol gradient sedimentation of crude mitochondrial extracts
revealed that TUTase activity associates with both 19S complex I and
35S-to-40S complex II (Fig. 1). By using an assay, we found that both
complexes contained single- and multiple-U addition activities when
poly(A) RNA was used as a substrate. However, we found that both of
these complexes added predominately a single U to gRNA substrates (Fig.
3A and data not shown). TUTase activity may be present in the upper
gradient fractions that correspond to ~10S (fractions 13 to 15), but
nucleases within these same fractions would mask such activity (Fig.
1).
When isolated mitochondria are incubated in the presence of
[-32P]UTP, editing complexes are labeled
(18-20). This labeling is the result of TUTase activity and
not mitochondrial transcription (13). We found that two
major RNP complexes became labeled during [-32P]UTP
incubation (Fig. 2). Based on prior studies, it is likely that these
two UTP-labeled complexes represent editing complexes I and II
(20). Those studies suggested that complex I functions as a
gRNA maturation complex that mediates the formation of the poly(U)
tail. This proposal was based on the colocalization of TUTase and
gRNAs, but not mRNAs, within complex I. However, the ability of complex
I to polyuridylate gRNAs was not examined. In our initial studies, we
found that the TUTase present in complex I could add only a single U to
three different gRNAs.
It has been shown that [-32P]UTP incorporates into
both mRNA and gRNA in isolated mitochondria (13, 18). In the
experiments described here, we evaluated the lengths of the labeled
gRNAs. We found evidence that complex II gRNAs are able to receive
approximately 15 U residues, the average length of a gRNA poly(U) tail.
Pulse-chase analysis of complex II gRNAs showed that the U tails were
added rapidly (within 5 min) and appeared to be stable throughout the experiment. In contrast, gRNAs associated with complex I did not increase significantly in size during the time course. These
experiments suggested that the addition of a 3' poly(U) tail to gRNAs
occurs within complex II.
Complex I TUTase from the glycerol gradient seems to have very
stringent nucleotide specificity for U. This result reinforced the
evidence that we were studying a TUTase and not a poly(A) polymerase or
another contaminating polymerase. An interesting product in these
assays was ligated RNA, which became readily detectable when ATP was
added. Self-ligated circular gRNAs were the prominent ligation product
(Fig. 1), since the 5' and 3' ends are in close proximity to each other
in the secondary structure of the gRNA (24). Circular gRNAs
were formed when we used 5'-end-labeled gRNA, due to the presence of a
5' monophosphate on this RNA. Neither uniformly labeled gRNA from T7
runoff transcriptions (which contains a 5' triphosphate) nor 3'-labeled
gRNA [which contains a 5' OH from poly(A) polymerase addition] would
produce these circles (data not shown).
A gRNA substrate that a priori contains a single 3' U nucleotide is not
a substrate for the addition of a second U (Fig. 3C). This result
eliminated the possibility that the single U addition was the result of
limiting amounts of a distributive TUTase. It is possible that the 19S
TUTase prefers to add a single U to an RNA that does not already
contain a 3' U. A TUTase that prefers to add a single U has been
described, although the activity on an RNA that a priori contains a
single 3' U nucleotide was not examined (29). Alternatively,
what appears to be a single U addition may be the result of competing
multiple-U-adding TUTase and 3' U-specific exonuclease activities. In
this scenario, an RNA that contains a single U would be a poor
substrate for the exonuclease. Recently, it was found that RNase E from
E. coli would trim back 3' poly(U) tails to leave a single
nucleotide uridylate remnant (14).
On glycerol gradients, we found that the single-U addition activity
cosedimented with the purified 19S complex. This finding suggests that
this TUTase activity is part of complex I (Fig. 1 to 4). However, we
have not analyzed whether our purified complex contained either gRNAs
or mRNAs, and it is possible that other factors were stripped away
during the purification. Multiple-U extension activity appears to
dissociate from the 19S complex, and treatment of the purified 19S
complex with a high salt concentration increases the amount of
multiple-U addition products (data not shown). At this stage, however,
we cannot exclude the possibility that the multiple-U addition TUTase
activity is a different TUTase also present in the 19S fraction which
is masked by the U-specific exonuclease during purification. Clearly,
these results warrant further investigations into how TUTase assembles
into 19S editing complexes.
In an effort to reconstitute gRNA polyuridylation, we sought conditions
that would shift the gRNA n+1 product to gRNAs containing a poly(U)
tail. The addition of ATP along with UTP did not promote gRNA
elongation, nor did the presence of a nonhydrolyzable ATP analogue
(AMP-CPP) inhibit gRNA n+1 TUTase activity. Since gRNAs interact with
mRNAs and our mitochondrial metabolic labeling results showed gRNA
poly(U) extension to occur in complex II, where mRNA is present, we
examined whether gRNAs could be polyuridylated when complexed with
cognate pre-mRNA (Fig. 5). Cognate pre-mRNA, but not noncognate
pre-mRNA, was sufficient to promote multiple-U tail formation.
Presumably, the 5' anchor of the gRNA would act to specify the
interaction with its cognate mRNA. However, we have not excluded the
possibility that the purine-rich regions of other noncognate pre-mRNAs
can stimulate gRNA poly(U) tail addition. One might expect that higher
concentrations of noncognate mRNA are required to produce the same
effect, although we have not tested this possibility.
Previous studies suggested that the poly(U) tail of the gRNA interacts
with the pre-edited region of the mRNA (6, 17). Our data
suggest that interaction of the newly synthesized poly(U) tail of the
gRNA with the purine-rich region of the mRNA protects the gRNA 3' tail
from editing complex-associated 3' U-specific exonuclease activity.
Alternatively, it is possible that the purine-rich region is required
for association of the gRNA with the editing complex and that the
association of gRNA with the editing complex, and not pre-mRNA,
protects the poly(U) tail from riboexonucleolytic trimming. It would be
very interesting if polypurine-rich RNAs were preferred RNAs for
association with editing complexes, since the polypurine-rich regions
are common at editing sites. However, the exact RNA preferences (if
there are any) that govern association with either the 19S or
35S-to-40S editing complex are not known. By changing the purine-rich
region to a pyrimidine-rich region, we abolished its ability to base
pair with the poly(U) tail. Interactions between the gRNA 5' anchor and
the mRNA do not seem to be critical for protection of the poly(U) tail,
since both RY and wild-type mRNAs contain the same 5' anchor. It is
more likely that the 3' U-specific exonuclease prefers a
non-base-paired nucleotide and that duplexing of the poly(U) tail
protects from exoribonucleolytic trimming.
How does the single-U addition activity present in the 19S complex
relate to mRNA editing? One possibility is that editing occurs through
multiple rounds of single-U addition and deletion, even at sites where
many U residues must be added or deleted (4). We have found
that the purified 19S complex is capable of performing U addition
editing and that predominately a single U is added to exogenously
supplied mRNA 5' cleavage fragments (data not shown). A second
possibility is that U addition to mRNA 5' cleavage fragments is similar
to the mRNA-dependent gRNA U addition described in this report. In this
possibility, multiple U residues would be added, which would then base
pair with the guiding nucleotides of the gRNA. Base-pairing
interactions would then protect the newly added U residues from
U-specific exonuclease.
These results support a model in which gRNA maturation occurs in
complex II (Fig. 7). gRNAs that are
associated with complex I are subject to both U addition and
riboexonucleolytic trimming. These gRNAs would contain a stable 3' U
residue. Upon assembly of complex II and prior to editing, these gRNAs
would receive multiple added U residues which would be stabilized by
the purine-rich regions of the pre-mRNA.
View larger version (19K):
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|
FIG. 7.
Proposed model of gRNA maturation. (A) gA6-[14] gRNA
with and without a poly(U) tail shown hybridized to the cognate
pre-mRNA substrate A6U2. The brackets represent gRNA anchor sequences.
(B) Model of complex assembly and gRNA maturation. gRNA is thought to
associate with complex I, where one U may be added at the 3' end. The
cognate mRNA may then associate via the gRNA anchor sequence,
disrupting the secondary structure of the gRNA. U residues are then
added to the gRNA, which form base pairs with the purine-rich region of
the pre-edited region. The pre-edited region of the mRNA is represented
as a box.
|
|
| |
ACKNOWLEDGMENTS |
We thank Robert Sabatini, Susan Madison-Antenucci, Mike Miller,
Karen Bertrand, and Jayleen Grams for helpful discussions and
insightful advice.
This work was supported by PSA grant CA 60151 to B.K.A. and PHS grant
AI 21401 to S.L.H.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biochemistry & Molecular Genetics, University of Alabama at Birmingham, Birmingham, AL 35294. Phone: (205) 934-6033. Fax: (205) 975-2547. E-mail: shajduk{at}bmg.bhs.uab.edu.
| |
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Molecular and Cellular Biology, February 2000, p. 883-891, Vol. 20, No. 3
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Top
Abstract
Introduction
