by an electrophoretlc mobillty. shlfE or by a change in the HPLC retention time of the 5r- phosphate versus the 5r-hydroxyl species. This requires an additional.
Tetrahedron Letters,YoI.27,No. Printed in Great Britain
0040-4039/86 $3.oo + .oo P e r g a m o nJ o u r n a l s L t d .
39,pp 4705-47O8,1986
CHEMICAL 5' -PHOSPIIORYLATIONOF OLIGODEOXYRIBONUCLEOTIDES THAT CAN BE MONITOREDBY TRITYL CATION RELEASE
Thornas Horn and Mlckey
Chiron Research Laboratories,
S. Urdea'
Chiron Corporation,
Eneryvllle,
4560 Horton Sgreet,
CA 94608, USA
ABSTMCT: A new phosphoramidite-derived -O-4,41reagent, (2-cyanoethoxy)-2-(2r dinethoxytrityloxyethylsulfonyl)ethoxy-NrN-dilsopropylaminophosphine, for the 5,phosphorylation of oligodeoxyribonucleotides has been developed. Phosphorylation efflciency can be deEermined by the release of 4,4r-dinethoxytrltyl catLon in acld. 5r-Phosphorylation the
5r-hydroxyl
Ehis
ls
forrn is
conducted
Alternatively,
versus
purificaclon retenElon
of tlme
mobillty
between the
the coupllng synthesized
shlfE
This
for
phosphorylaElon
a phosphorylatlon cation is
reagents reactlon.
is
usually
as
Usually kinase.
fully
of
protected
Ehat employ
Also, for
afEer
acld
WheEher or not
an additional
polynucleoEides
(1)
purlficatlon
time of
the 5r-
and
1n Ehe rnobllity larger
or
than 20 bases.
be monitored
deprotection
that
the 5r-
after
work-up
che difference
deEermlned.
DMTCi DMT-OCH2CH2SO2CH2CH2 OH PYRIDINE
to dage is
determined
reagenE Ehat could
tradltionally
reported
the HPLC retention
requires
ollgoner.
Ewo forms ls minimal
DNA synthesis
applications.
ATP and To polynucleotide
or by a change in
species.
lhe unphosphorylated
HO CH2CH2SO2CH2CH2-OH
wlth
trrost chernical phosphorylaelon
the 5r-hydroxyl
durlng
ollgoners
which are syntheslzed
biologlcal
chemisEry (2).
the orange 4,4r-dfunethoxytrityl
nucleotldes
molecular
can be used on automated DNA synuhesizers
way to rnonltor
We chose Eo deslgn of
for
have been developed
fragrnent was actually
by an electrophoretlc phosphate
purlfled
phosphoramldite
no convenient
phosphorylated
oligodeoxyribonucleotldes
necessary
by treaLing
One drawback ltith ls
often
sorne of which
solid-supporced
there
synthetic
chernlcal nethods
(lr2),
fragments
of
by the release
the same way coupling
of
A1so, we were interesEed
ln
R = COCH2CH2CO NH CPG R'=H
ruco-r2cu2o-e-r( 14 ct
R
_1 OIPEA
DMT-O-CH2CH2SO2CH2CH20. TR P.N 'R NCCH2CH2O'
(3)
O B O B R =,P-o+---, F o ,,l-o cocx2cn2co'NH cPG o-cHs o,cH3
R= - 9 H c H 3 CH: B HO+OR '
,r,
Q
B
R= Po+ o" ====+=:TFTRAZoIF
A
q
o-P-o+oH o-
DMTO.CH2CH2SO2CH2CH2O.B P.OrrOR NccH2cH2o €)
D M T O C H 2 C H 2 S O 2-C H -'F-o1on 2CH2O\:?^B^^. NH4OH NCCH2CH2O
O
B
=oo|f,; oPotoq O-
Scherne I
4705
(4)
tt
,
LUTTD|NE
NH4oH 60"C.18h
o i o,lt o* o_
4706
fully
reagent
the
naklng
Since removal
of
protecting
of
more rigorous
requires
(4).
co hydrolysis
resistan!
being parlicularly
protecting
potenlial
Another
possible
is
phosphate diesters
in
former
the
in
protection
ether-conlaining
to our needs appeared to
be tailored
by Tesser et al
(5,6).
As for
the 2groups from
and arylsulfonylethyl
alkyl-
of both
compleEe elimlnation
function,
cyanoechyl
elirnlnated
thaE could
function
group reported
be rhe alk(ar)ylsulfonylethyl
(2)'
from a phosphate diester
these funclions'
of
phosphorus based on elther
scheme for
can be --
groups that
protecting
a trityl
to derive
would however be difficult
It
NH4OH.
can be fully
it
since
attractive
are particularly
have proven useful
and p-nitrophenylethyl
such as 2-cyanoethyl
eliminated
the choice
deprotecEion,
phosphate diesters
Ehis reason that
for
forrn Cypically
fhe diester
agents has been an important
and sirnple alkyl
is
It
in
triesEer
than {nternucleotide
aromatic
Halogenated
consideration.
from phosphate
phosphorylating
for
These
groups where one
blocking
a dialkylaminophosphine.
functions
conditions
groups
blocking
suiEable
for
ether
a dimethoxytrityl
(3).
chernlstry
s u g g e s L e d t h e u s e o f a s e E o f N H 4 O T {s e n s i l i v e
requirenents carries
phosphoramidite
with
compatible
N H O O Hs o l u t i o n .
Thus, we designed and prepared (2-cyanoethoxy)-2'(2r-4,4'-dirnethoxyltiLyloxy and tested
ethylsulfonyl)eChoxy-N,N-diisopropylaminophosphine(3) (Scherne I).
reagent
To solid
standing.
in
stirring
chloride for
the dark
dissolved
residue
in
ethyl
phase was dried
the producE was purified
solvents
by silica
gel
was left in
was then concentrated
(500 n1) was extracted
acetate
(150 m1) was added
pyridine
50 rnrnole)and the mixture
solution
The reacEion
l8h.
on
which crystallized
58.6 nmole) in
(DMT-CI; I6.95 g,
aq. NaCl and the organic
salurated
(10.6 g,
sulfonyldiechanol
4,4'-dimethoxyrrityl
oil
to give a viscous
dry acetonitrile
with
coevaporation
by repeated
in HrO) was dried
(65% w/v
sulfonyldiethanol
available
Commercially
of
as a phosphorylatlon
it
with
The
vacuo.
5 % a q . N a H C O 3a n d 8 0 2 rernoval
After
over anhydrous Na2S0O'
10.0 g of
column chromatography to give
purel(TLC,si1lca]rnCH2CI,;Rf=o.015).Ch1oro-N,N-diisopropylarnino-2-cyanoethoxysolution of I (4.5 phosphine 2 (4.6 mrnole) was added rapidly under argon to a stirred (10 rn1) at (DIPEA; 4.6 mnole) in rnethylene chloride mnole) and N,N-diisopropylethylarnine acetate (50 w i L h e t h y l 0 C. The solution was allowed to warm to room temperature, diluted nl)
and washed with
acetonitrile
and then
(2 x 20 n1).
into
aliquoted
The organic
1.5 rn1 septum-sealed
was removed by evacuatlon
added to a detritylated iodine 90 sec.
and thorough
spectroscopy suggesting at
a coupling
NMR sEudles
indicated
collected
efficiency
2O C and the supernatant
obtained
of
96%.
synthesis
of
and
$7lth aqueous
5Z w/v DCA in
Cl{rCl,
for
absorption
the original
thymidine
support
was exposed to 2 m1 of NH4Otlfor 2h 3IP5h. TLC, HPLC..rd an additional
The polyner
was healed at 60 c for
quantitative
2 mL of
of
under
Purlfication. in dry acetonitrile
was compared by visible
from deprotection
each containing
was stored
sEandard oxidatlon with
Ehe supporE was treated
orange solution
to the naterial
After
C?G support.
thyrnidine
washing,
The brighC
0.75 ml of 0.5 M lH-teerazole
with
with
was dissolved
Wheaton vials
and the product
The solvent 100 {mo1e of 3. .argon at -2O C (7). This crude product was used $rithouc further Reagent 3 was activated
phase was dried
product
The oily
evaporation.
by rotary
N a T S O Oa n d c o n c e n t r a t e d
anhydrous in
aq. Nacl
8oz saturated
thymldine
5'-monophosphate
without
4707
TABLE I.
Conpound
sol
T
Ho+oH 9 r Ho,?o+oH H
o
o
r
"u.o[,oio" rio.j-oa no
ra
sol
(R- :min)
rra
o'90
o'77
1'66
0.59
0.14
0.67
0.69
0.29
1.84
0.70
0.30
l.l0
o r our-o.esr-o,F,o.l-on ieo-'-
a ) N H a o H , 2 o . 0c . 5 9 , 0 . 6 9 ' b)NH4oH,6ot
0.59
g i -O+OH oMT-O.ESE,O.f cE.o
a)NHaoH,2o.c
N.D.
b )N H 4 o H , 6 o ' c
0.70-
3lp-Nlg"
HPLcb
T L C' (Rr. )
0.33',0.29,0.14
( oom)
4.01 +0.7(pyridinium salr)d -6.0,-5.9(Nnf-sa1t)d
I.94,O.67
0.14
0.67
N.D.
4.10,4.50
0.22"
0.70
N.D. 4.025 N.D.
a
_43.25
cE - NCCH2CH2. ESE--CH2CH2SO2CH2CF12. a) Sol I and Sol 7.5, respectively;
(v/v) are 8:2 and 9:l b) Cl8 reverse phase;
II
isopropanol: 0.1 M Triethylanrnonium 2.5 to l)'i( CH"CN in 0.05 M NH/HrpO/,
c) relarive 8.8; (10) d) DTNB in I M NMR spectrum
ro I M H"Po, in D"o; measured in Dro,"reTative'to H.Po4; e) Tris,-pH 8.0; f) DI"ffp5sitive was obEained if detritylation
concomitant
producEion of phosphonate or partially
When deprotection only,
a mixture
thyrnidine
If
5t-phosphorylated
sulfur
? l
evidenced by'^P-NMR
for
(f0).
naleirnido-
(the
of
to
Lhe 5'-phosphorothioate
coupling
efflciency
purlfied kinase
The use of permils
phosphorus
a low coupling. unmasking of phosphorylation investigatlng
Although
a new hydroxyl is other
of T4 DNA ligase
easily sinilar
the material
Thus lt
by the lack
is
of startlng
noiety
not
that
ideal
Ehe side-product
since
obtained
protecting
with
by
was deprotected
and
T4 polynucleotide
the chemically
if
and
ligatlon. reporEed here concomitant
rnoniloring results
in
reveals the
an additional
upon irork-up.
groups for
(12).
to check the
after
reaction
detritylation
and
Both sequences are near
materlal
the
as
on an automated
can be removed without
to repeat
removed frorn the oligonucleolide blfunctional
l.
I)
manner.
chemistry
group such as sulfonyldiethanol
possible
compound I is group,
lhis
k'ith
using
Figure
(8).
exchange can be
3, detritylated
reactions
are presenced in
protecting
of a noniEoring
deprotection.
of
(tabl.e
Solid-supported
phosphoranidite
reagent
The second half
fragments
as evidenced
a bifunctional
che introduction
(11).
The producE was then purified
deprotected.
The PAGE analyses
phosphorylated
fully
and disulfide
forrn which was then 5r-phosphorylated
phosphorylated
enzyr:natically
rrith
60 C NHaOH was obtained
a reasonably good
ls
sequence GGATCCGGATC wC as synthesized
electrophoresis.
as the 5r-hydroxyl and ATP.
reagents
at Ehis functlon
was phosphorylated
20 C
the 5r-phosphltylated
probes have been produced in
oligonucleotide
and fu1ly
gel
with
derlvative
in phosphorothioates
speciflcally
BarnHI linker
Lhe support
step (9),
converted
Geno-O-Matlc) using a solid-supported
One-half
polyacrylarnide
\.ras deprotected
the oxidation
and bromoacetyl-concaining
N H 4 O Ha t
and 2-cyanoethyl-5r-phosphate
in
Slnce the sulfur
labeled
The palindrornic instrument
was conducted with
iodine
used to modify oligonucleo!ides non-radioactively
thymidine
(Table I).
nucleotide
a mixEure of both 5r-phosphonate and nucleoslde
was quantitaLively
nucleophile,
protected
thymidine
5r-phosphitylated
oxidation,
By substltuting thymidine
in 502 D,o add 507. I v1 Tris-frc1-0105M ED'|A, pH becomes'bright ye11ow when sprayed with l0 mM a s e v i d e n c e d b y 1 0 7 "H ' S O , s p r a y ; g ) a n i d e n t i c a l was perforrned prior to NIIooH treatnent.
of boEh 2-(2r-hydroxyethylsulfonyl)ethyl-
was noted.
prior
without
of
pH
acetate pH 4.0;
We are
chernical phosphorylatlon
