Treatment of murine L1210 lymphoid leukemia and melanoma B16 with lipophilic cytosine arabinoside prodrugs incorporated into unilamellar liposomes

Rubas, Werner; Supersaxo, A.; Weder, H. G.; Hartmann, H. R.; Hengartner, Hans; Schott, Herbert; Schwendener, Reto A.

doi:10.1002/ijc.2910370123

Cited by 65 publications

(27 citation statements)

References 16 publications

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“…For the cytotoxicity experiments liposomes with the same lipid composition were used but NOAC was added at 20 mM (1500 molecules NOAC per liposome). For the flow cytometry experiments liposomes with the same lipid composition, 1 mM DiI and 180 mM sodium cholate were prepared by dialysis against saline-EDTA as described by Rubas et al (1986). DiI concentration was determined with a Spectrofluorometer SFM 23 (Kontron, Zurich, Switzerland) after solubilization of an aliquot of liposomes (20 µl) with 2 ml sodium cholate (0.05%), yielding an average of 80 DiI probes per liposome.…”

Section: Preparation Of Liposomesmentioning

confidence: 99%

Low density lipoprotein and liposome mediated uptake and cytotoxic effect of N4-octadecyl-1-β-D-arabinofuranosylcytosine in Daudi lymphoma cells

1999

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Summary Low density lipoprotein (LDL) receptor-mediated uptake and cytotoxic effects of N 4 -octadecyl-1-β-D-arabinofuranosylcytosine (NOAC) were studied in Daudi lymphoma cells. NOAC was either incorporated into LDL or liposomes to compare specific and unspecific uptake mechanisms. Binding of LDL to Daudi cells was not altered after NOAC incorporation (K D 60 nM). Binding of liposomal NOAC was not saturable with increasing concentrations. Specific binding of NOAC-LDL to Daudi cells was five times higher than to human lymphocytes. LDL receptor binding could be blocked and up-or down-regulated. Co-incubation with colchicine reduced NOAC-LDL uptake by 36%. These results suggested that NOAC-LDL is taken up via the LDL receptor pathway. In an in vitro cytotoxicity test, the IC 50 of NOAC-LDL was about 160 µM, whereas with liposomal NOAC the IC 50 was 40 µM. Blocking the LDL receptors with empty LDL protected 50% of the cells from NOAC cytotoxicity. The cellular distribution of NOAC-LDL or NOAC-liposomes differed only in the membrane and nuclei fraction with 13% and 6% respectively. Although it is more convenient to prepare NOAC-liposomes as compared to the loading of LDL particles with the drug, the receptor-mediated uptake of NOAC-LDL provides an interesting rationale for the specific delivery of the drug to tumours that express elevated numbers of LDL receptors.

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Section: Preparation Of Liposomesmentioning

confidence: 99%

Low density lipoprotein and liposome mediated uptake and cytotoxic effect of N4-octadecyl-1-β-D-arabinofuranosylcytosine in Daudi lymphoma cells

1999

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“…A third technique involves the modification of hydrophilic drugs into lipophilic derivatives (prodrugs). These molecules are incorporated as lipophilic components into the liposomal membrane (Rahman et al, 1986;Rubas et al, 1986).…”

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confidence: 99%

Comparative pharmacokinetic and cytotoxic analysis of three different formulations of mitoxantrone in mice

Rentsch

Horber²,

Schwendener³

et al. 1997

Br J Cancer

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MTO, 6.1 imol kg-' for PA-MTO and 4.5 Imol kg-' for pH-MTO. The concentrations of MTO were determined using high-performance liquid chromatography (HPLC) in blood, liver, heart, spleen and kidneys of the mice. Additionally, the toxicity and anti-tumour activity of MTO was evaluated in a xenograft model using a human LXFL 529/6 large-cell lung carcinoma. The dose administered was 90% of the maximum tolerated dose (MTD) of the corresponding formulation (8.1 Amol kg-' for free MTO, 12.1 iimol kg-' for PA-MTO and pH-MTO). The pharmacokinetic behaviour of PA-MTO in blood was faster than that of free MTO, but the cytotoxic effect was improved. In contrast, pH-MTO showed a tenfold increased area under the curve (AUC) in blood compared with free MTO, without improvement of the cytotoxic effect. This discrepancy between the pharmacokinetic and cytotoxic results could be explained by the fact that MTO in pH-MTO liposomes remains mainly in the vascular space, whereas MTO in PA-MTO liposomes is rapidly distributed into deep compartments, even more so than free MTO.

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“…PC, 15-3 Bq/mmol) and manganese chloride (54MnC12) were from Amersham Int, Amersham, U K N2-Palmatoyl-L-lyslne methyl ester HC1 (PL) was synthesized as described [15] The hpopinhc malelrmde derivatives N 6-(3-malelmldopropmnyl)phosphaudylethanolarmde (MP-PE) and N6-(6-malemudocaproyl) -phosphaudylethanolarmne (EMC-PE) were prepared m analogy to the pubhshed synthesis of N-(4-(pmalelrmdophenyl)butyryl)phosphatldylethanolamlne [4] N4-Oleyl-ara-C (NOAC) was prepared as described before [17] and the hpophlhc metal complexmg agent DTPA-stearate as described in Ref 19 The Inghly fluorescent hpophlhc perylene dye N, N'-bls(1-hexylheptyl)-3,4 9,10-perylenebls(dlcarboxlmlde) (BHPD) was obtained from 7-trxdecanamlne as described before [20] Before use BHPD was purified on a Sdlca-gel column with CHC13 as eluent N-Succlnlmldyl-S-acetylthloacetate (SATA) was prepared according to Ref 21 …”

Section: Palmltoyl-l-3-phosphatldyl[ N-methyl-3h]chohne (3h-mentioning

confidence: 99%

“…Small undamellar llposomes were prepared by detergent dialysis as descnbed before [17] The matrix hpld composmon used throughout all hposome preparations was soy phosphatldylchohne (SPC)/cholesterol/DL-atocopherol at 1 0 2 0 01 mol parts with 20 mg SPC/ml (26 #mol/ml) lmtml hpld concentration The malemude derlvatwes MP-PL, MP-PE, EMC-PL and EMC-PE were added at 0 02 or 0 05 mol parts Nn-oleyl-ara-C (NOAC) concentraUon was 0 2 mol parts The hpophlhc fluorescent label BHPD was Incorporated at 0 006 mol parts into the hposome membranes All hplds Including the corresponding malelnude denvatwe plus NOAC and BHPD were dissolved in MeOH/CHC13 (1 1, v/v) Sodmm cholate as detergent was added at a ratio of 0 6-0 7 moles referred to the sum of the concentraUons of all membrane-fornung hplds In some preparations the llposomes were labeled by addmon of trace amounts of 3H-PC or by the mcorporaUon of 0 003 mol parts of the hpopluhc chelating agent DTPA-SA to which radioactive manganese (54Mn2+) ions were complexed after hposome formation [19] After the removal of the orgamc solvents on a rotatory evaporator (40 o C, 60 rmn) the hpld/detergent nuxtures were solub~hzed by addmon of phosphate buffer (67 mM dlsodmm hydrogen phosphate dlhydrate/67 mM potassium dlhydrogen phosphate (pH 7 4)) The resulting nucellar solutions (10-20 ml) were dialyzed against 5-10 1 of the same buffer at 40°C for the first 2 h, followed by dialysis at 25 °C for another 24-36 h The hposome preparations were filtered through 0 45 #m sterile filters (Sartonus) and stored at 4 o C Llposome s~zes and homogeneity were deternuned by laser light scattering and negattve stare freeze-fracture electron microscopy [17] The mean number of membrane-fornung molecules, wluch comprised all hpopluhc compounds constituting the membrane bdayer of one hposome and the total number of hposomes formed by the hpld concentraUon umt of 1 mg SPC/ml, were calculated from the mean vesicle diameters obtaaned from the laser hght scattenng data and from the assumptions on vesicle geometry parameters as made by Huang …”

Section: Preparatton Of N4-oleyl-ara-c Hposomes Containing Vartous Hpmentioning

confidence: 99%

“…The covalent couphng of Abs, Ab fragments or peptldes to hgands winch are located on the surface of hposomes can be achieved by numerous chemical methods [3][4][5][6][7][8][9][10][11][12][13][14][15][16] Bffunctmnal hgands have become useful tools for the couphng of proteins to hposomes Among a vanety of such molecules, N-succlmmldyl-3-(2-pyndyldlthlo)propinnate (SPDP) is currently one of the most used linkers, although ~t has a number of disadvantages hke its suscept~inhty to traces of reducing agents and the short half-hfe of the reactwe sulfhydryl groups [16] N-Succxnlrmdyl-S-acetyltinoacetate (SATA) is an alternatwe couphng agent [16] In tins work we present the results that were obtained by the direct comparison of Ab couphng methods using SPDP and SATA as hnkers to hposomes which contmned N4-oleylcytosme arabmoslde (NOAC), a hpopinhc denvatwe of arabmosylcytoslne, as cytostatic prodrug [17,18] In particular, the couphng of the two Abs, B8-24 3 specific for the mouse MHC class I H-2k b surface antigen on EL4 mouse T lymphoma cells and IB16-6, specific for a surface antigen on B16 mouse melanoma cells, to small umlamellar drug carrying hposomes was lnvest~gated In addmon, the new highly fluorescent hpopinhc dye N,N'-b~s(1-hexylheptyl)-3,4 9,10-perylenebls(dlcarboxlnude) (BHPD) was used as fluorescence label for the hposomes…”

Section: Introductionmentioning

confidence: 99%

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Comparative studies of the preparation of immunoliposomes with the use of two bifunctional coupling agents and investigation of in vitro immunoliposome-target cell binding by cytofluorometry and electron microscopy

Schwendener¹,

Trüb²,

Schott³

et al. 1990

Biochimica et Biophysica Acta (BBA) - Biomembranes

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The two coupling agents SPDP (N-succinimidyl-3-(2-pyridyldithio)propionate) and SATA (N-succinimidyi-Sacetylthioacetate) were compared in their efficiency and feasibility to couple monocional antibodies (Abs) via thioether linkage to liposomes functionalized by various lipophilic maleimide compounds like N-(3-maleimidopropionyl)-N2-palmitoyi-L-lysine methyl ester (MP-PL), N-(3-maleimidopropionyl)phosphatidylethanolamide (MP-PE), N6-(6-maleimidocaproyl)-N2-palmitoyI-L-iysine methyl ester (EMC-PL), and N-(6-maleimidocaproyl)phosphatidylethanolamine (EMC-PE). The composition of the iiposomes was soy phosphatidylcholine (SPC), cholesterol, maleimide compounds and a-tocopherol (1:0.2:0.02:0.01, mol parts), plus N4-oleyicytosine arabinoside (NOAC) as cytostatic prodrug (0.2 mol parts) and a new, lipophilic and highly fluorescent dye N,N'-bis(1-hexylheptyl)-3,4:9,10-perylenebis(dicarboximide) (BHPD, 0.006 mol parts). From the maleimide derivatives MP-PL was the most effective in terms of preservation of the coupling activity in dependence of iiposome storage. The coupling of the monoclonal A B8-24.3 (mouse IgG2b, MHC class I, anti H-gk b) and 11316-6 (rat IgG2a, anti B16 mouse melanoma) to the drug carrying liposomes was more effective and easier to accomplish with SATA as compared to SPDP. Coupling rates of 60-65% were obtained with SATA at molar ratios of 12 SATA:I Ab:40 maleimide spacer groups on the surface of one liposome. The highest coupling rates with SPDP were obtained at the ratio of 24 SPDP: 1 Ab:40 liposomal maleimide groups, with an Ab binding efficiency of only 20-25%. The optimal in vitro binding conditions to specific target cells (EIA for BS-24.3-1iposomes and B16-F10 for IB16-6-1iposomes) were determined by cytofluorometric measurement of the iiposomal BHPD fluorescence with SATA linked Abs. Optimal immunoliposome binding to specific epitopes on the target cells was achieved with 1-2 Ab molecules coupled to one liposome, with immunoliposome concentrations of 20-130 nM and with a small incubation volume of 0.3-0.4 ml. The specificity of the binding of BS-24.3-1iposomes to EIA target cells was visualized by scanning electron microscopy. Antibody mediated endocytic uptake of immunoliposomes could be demonstrated by transmission electron microscopy.

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Treatment of murine L1210 lymphoid leukemia and melanoma B16 with lipophilic cytosine arabinoside prodrugs incorporated into unilamellar liposomes

Cited by 65 publications

References 16 publications

Low density lipoprotein and liposome mediated uptake and cytotoxic effect of N4-octadecyl-1-β-D-arabinofuranosylcytosine in Daudi lymphoma cells

Low density lipoprotein and liposome mediated uptake and cytotoxic effect of N4-octadecyl-1-β-D-arabinofuranosylcytosine in Daudi lymphoma cells

Comparative pharmacokinetic and cytotoxic analysis of three different formulations of mitoxantrone in mice

Comparative studies of the preparation of immunoliposomes with the use of two bifunctional coupling agents and investigation of in vitro immunoliposome-target cell binding by cytofluorometry and electron microscopy

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