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Blood, Vol. 91 No. 12 (June 15), 1998:
pp. 4738-4746
By
From the University Department of Haematology, Royal Liverpool
University Hospital, Liverpool, UK; and the School of Biological
Sciences, University of Liverpool, Liverpool, UK.
The hybrid gene BCR-ABL that typifies chronic myeloid
leukemia (CML) represents an attractive target for therapy with
antisense oligodeoxyribonucleotides (ODN). A central obstacle in the
therapeutic application of ODN is their poor cellular uptake. Adding
various lipophilic conjugates to the ODN backbone has been reported to improve uptake, and electroporation of target cells has also been shown
to enhance intracellular ODN delivery. We have shown that (1)
BCR-ABL-directed ODN will specifically decrease the level of
BCR-ABL mRNA, provided that cells are first permeabilized with Streptolysin-O (SL-O), and (2) chimeric
methylphosphonodiester:phosphodiester ODN directed against 9 bases
either side of the BCR-ABL junction are more efficient ODN
effectors than structures composed solely of phosphodiester or
phosphorothioate linkages. In this study, we compared the efficacy of
lipophilic conjugation, SL-O permeabilization and electroporation on
the intracellular delivery and molecular effect of
BCR-ABL-directed ODN. b2a2- and b3a2-directed chimeric ODN
were synthesized either unmodified or with one of the following groups
at the 5
IN CHRONIC MYELOID leukemia (CML), the
characteristic Philadelphia abnormality translocates part of the
ABL gene on chromosome 9q34 to the major breakpoint cluster
region BCR on chromosome 22q11.1 The resultant
hybrid gene BCR-ABL is leukemia-specific, and its protein
product (p210) is likely to be central in the maintenance of the
leukemic phenotype. BCR-ABL mRNA therefore represents an
attractive target for antisense oligodeoxyribonucleotides (ODN).
Several groups have reported their experience with short (18-26mer) ODN
on CML cells and cell lines.2-5 Most groups report that ODN
decrease p210 expression, BCR-ABL transcript level, or CML cell
growth in in vitro culture, although the effects may be
nonspecific.3,4,6 In these studies, all the constituent nucleosides have been either wholly phosphodiester (PO)-linked or
wholly phosphorothioate (PS)-linked. However, PO-linked ODN are highly
sensitive to nucleases present both intracellularly and in
serum.7 Furthermore, PS-linked analogues, although
significantly more resistant to nuclease degradation, may bind
nonspecifically to a variety of intracellular molecules, such as
nucleic acid polymerases,8 and PS-linked ODN may produce
nonantisense aptameric effects in CML cells.9,10 Apparent
positive results with PS-linked ODN may therefore be due to nonspecific
nonantisense effects,3 which may not be leukemia-specific
when mixed populations of leukemic and normal cells are studied.
ODN in which all the bases are linked by methylphosphonodiester (MP)
linkages are totally resistant to nucleases. All MP-linked ODN have
been used to target BCR-ABL mRNA,11 with reported
selective decrease in BCR-ABL p210 protein levels and an
antiproliferative effect. However, all MP-linked ODN are poorly soluble
and exhibit low affinity for their target mRNA. All MP-linked ODN are
also unable to direct destruction of target mRNA by RNase H, a
ubiquitous cellular enzyme that cleaves the RNA component of DNA:RNA
heteroduplexes.12 In the hope of combining useful
properties of both MP- and PO-linked ODN structures, we have therefore
designed novel MP:PO:MP chimeric ODN, consisting of terminal MP-linked
sections flanking a central PO-linked region
(Fig 1). The flanking MP linkages confer
protection against exonucleases, whereas the central PO-linked section
will retain highly specific cleavage of BCR-ABL mRNA by
targeting RNase H. We have shown in previous work that such chimeric
ODN have superior specific antisense properties and are more stable in cell extracts when compared with conventionally linked
ODN.13
A central problem in the application of ODN to living cells is their
poor cytosolic uptake.14,15 Reported antiproliferative effects from experiments in which ODN are simply added to the culture
medium may result from nonantisense mechanisms,16,17 and
this is especially true for wholly PS-linked ODN structures. Several
reports have suggested that introduction of lipophilic groups into ODN
structure will enhance intracellular delivery of ODN, with concomitant
increase in antisense efficacy. Introduction of a lipophilic dodecanol
chain18 or cholesterol19 at the 3 In the present work, we set out to compare these three different
strategies of improving BCR-ABL-directed ODN delivery to CML
cells: (1) SL-O permeabilization of target cells, (2) electroporation of target cells, and (3) conjugation of ODN with various lipophilic structures. We have examined their effect on ODN uptake and
intracellular localization and have investigated ODN delivered by these
techniques on inhibiting target mRNA expression.
ODN structure and synthesis.
All ODN structures studied were 18-mers, complementary to an 18-base
mRNA sequence spanning either the b3a2 or the b2a2 BCR-ABL fusion breakpoint (Fig 1). The overall structure was chimeric in
design, composed of 4MP:9PO:4MP internucleoside linkages. To assess
cellular uptake and intracellular localization, all ODN were labeled
with fluorescein. As well as unconjugated ODN, structures were studied
that were conjugated to one of the following lipophilic groups at the
5 Cells and cell lines.
The human b2a2 BCR-ABL-containing CML cell line KYO1 (generous
gift of Dr S. O'Brien, LRF Leukaemia Unit, Hammersmith Hospital, London, UK) was used as a target in which to study ODN uptake. KYO1
cells were cultured in RPMI 1640 medium supplemented with L-glutamine
(GIBCO Ltd, Paisley, UK) and 10% heat-inactivated fetal bovine serum
(FBS; Sera Lab, JRH Biosciences, West Sussex, UK). Cells were
maintained in logarithmic phase of growth by subculturing thrice
weekly.
Uptake experiments and flow cytometry.
All uptake studies were performed using purified ODN to ensure that
only intact oligonucleotide was studied. A total of 106
cells in 50 µL of RPMI/FBS were incubated with 20 µmol/L ODN at
37°C for up to 6 hours. Ten-microliter aliquots were removed at
intervals into 1 mL of RPMI/FBS containing 10 µg/mL of propidium iodide (PI) at 4°C for 10 minutes and washed three times in
RPMI/FBS. All experiments were performed in duplicate.
SL-O permeabilization.
The technique for SL-O permeabilization was essentially that of Barry
et al,29 modified as previously
described.24,25,30
Electroporation.
After washing once in RPMI, 5 × 106 KYO1 cells were
resuspended in 800 µL RPMI at 4°C. ODN was added where required
to give a final concentration of 20 µmol/L. The cell suspension was
transferred to ice-cold 0.4-mm gap electroporation cuvettes (BioRad,
Hemel Hempstead, Hertfordshire, UK), and cells permeabilized with a single pulse from a Gene Pulser attached to optional capacitance extender (BioRad) set to 960 µF, 250 V. These conditions were defined
as producing optimal permeabilization with minimal toxicity in
preliminary experiments and resulted in an electroporation time
constant of approximately 20 milliseconds. The cells were incubated for
60 minutes at 4°C in the electroporation cuvettes and then
transferred to flasks containing 10 mL of prewarmed gassed RPMI as for
SL-O permeabilization.
Transfection by Lipofectin.
ODN and 30 µL Lipofectin (GIBCO) were allowed to associate for 15 minutes at 37°C, using sufficient ODN to achieve a final concentration of 2 µmol/L after addition to the cell suspensions. This ratio of ODN:Lipofectin was defined in preliminary experiments as
that maximizing cell-associated ODN. KYO1 cells (5 × 106) were suspended in 200 µL RPMI, incubated with
ODN/Lipofectin mixture at 37°C for 15 minutes, and then transferred
to flasks containing 10 mL warmed gassed RPMI. No attempt was made to
remove the Lipofectin. The dose of ODN/Lipofectin used was the maximum dose that did not induce excessive acute toxicity (cell death <30%
at 4 hours, as measured by PI counterstaining).
RNA purification and analysis.
Total cellular RNA was prepared from samples of experimental cells by
the guanidinium thiocyanate-acid phenol method.31 RNA
precipitates were resuspended in deionized diethylpyrocarbonate-treated formamide,32 and their relative concentrations were
estimated by gel electrophoresis and ethidium bromide staining.
Denaturing agarose gel electrophoresis, transfer of RNA to Nytran nylon
membrane (0.2-µm pore; Schleicher and Schuell; UK distributor
Anderman and Co Ltd, Kingston-upon-Thames, Surrey, UK), hybridization
to digoxigenin-labeled probe, and subsequent chromogenic visualization procedures were all performed as previously described,33
except that digoxigenin-labeled antisense RNA was used as
probe34 rather than random-primed DNA. The blots were
quantified using a Shimadzu CS9000 flying spot densitometer (Shimadzu;
UK distributor Howe and Co Ltd, Banbury, Oxfordshire, UK), as
previously described.35 The expression of BCR-ABL
and irrelevant control (C-MYC, p53, and
glyceraldehyde-3-phosphate dehydrogenase [GAPDH]) mRNAs were corrected for the flow cytometrically determined number of cells from
which the RNA was extracted. Results are expressed as relative to an
untreated control.
ODN uptake.
Figure 2 gives the ODN uptake into KYO1
cells exposed continuously to b2a2-directed ODN of various structures
for 6 hours. All ODN were used at a concentration of 20 µmol/L,
except for ODN conjugated to cholesterol or vitamin E, which were used
at a concentration of 2 µmol/L, because higher ODN concentrations caused lysis of target cells because of membrane damage. Uptake is
expressed as the log of attomoles of fluorescein-labeled ODN per cell.
No difference in ODN uptake is seen for conjugated structures in
comparison with unconjugated ODN. Similarly, no difference was seen for
ODN associated with Lipofectin (data not shown). For ODN directed
against the b3a2 junction, the same pattern and level of uptake was
seen (data not shown).
Effect on mRNA expression.
Figure 5A shows the effect of various ODN
structures on the expression of BCR-ABL mRNA in KYO1 cells, 4 hours after a pulsed exposure to ODN. No structure decreased mRNA
expression to less than 80% of that of an untreated control. ODN
associated with Lipofectin had no effect (data not shown). No
consistent difference was seen between the effect of b2a2- and
b3a2-directed ODN. No ODN (whether b2a2- or b3a2-directed) decreased
the expression of p53, C-MYC, or GAPDH mRNA
(data not shown).
Cellular localization of ODN.
Figure 6 shows a series of fluorescence
microscopic appearances of KYO1 cells after exposure to ODN. Figure 6A
shows the appearances with 100 µmol/L 4-9-4 chimeric ODN, without
SL-O permeabilization. There is a vesicular intracellular distribution,
compatible with uptake by fluid phase pinocytosis. Similar appearances
were seen with ODN conjugated with POE, Dodecanol, and PEG2 or PEG5,
with no evidence of improved intracellular delivery.
Although leukemic cells may take up ODN more readily than normal
cells,36 for ODN to have a worthwhile biological effect, some means of enhancing cellular uptake is essential. As a prelude to
clinical studies of ODN for purging hemopoietic cell harvests from
patients with CML, we have examined three different strategies for
improving the effectiveness of ODN in CML cells. The present data again
demonstrate the lack of significant intracellular ODN uptake and
molecular effect if ODN (of whatever structure) are simply added to
cells. We report that SL-O permeabilization or electroporation of
target cells is superior to lipophilic conjugation or Lipofectin
association for improving intracellular ODN delivery, achieving levels
of approximately 5 to 10 and 1 attomole respectively per cell. The
approximately 0.1 to 1 attomole per cell achieved with a variety of
conjugated structures without prior permeabilization of target cells is
comparable with that observed by Smetsers et al4 using 10 µmol/L PS-linked 26-mer ODN without uptake enhancement in BV173
cells, also a b2a2 BCR-ABL-containing cell line. The fluorescence micrographs demonstrate that the cellular distribution of
ODN is predominantly intranuclear after SL-O permeabilization or
electroporation, in contrast to the surface membrane and vesicular localization seen for conjugated structures. The superior uptake and
cellular localization seen with SL-O permeabilization and electroporation translates into increased biological effectiveness, as
evidenced by the decreased target mRNA levels, not seen in unmanipulated target cells treated by conjugated or
Lipofectin-associated ODN structures.
Submitted June 3, 1997;
accepted February 12, 1998.
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e |
Abstract
Introduction
end: cholesterol, vitamin E, polyethylene glycol of
average molecular weight 2,000 or 5,000, N-octyl-oligo-oxyethylene, or
dodecanol. ODN associated with Lipofectin was also studied. Comparison
was made in untreated, electroporated, and SL-O permeabilized KYO1
cells. Uptake was examined by fluorescence microscopy and flow
cytometry, using ODN structures that were 3
Abstract
20°C in the dark
until use.
) 2 µmol/L 5
) 20 µmol/L
5
) 20 µmol/L 5
) 20 µmol/L
5
) 20 µmol/L
5
) 20 µmol/L 5
