α<sub>2</sub>‐Macroglobulin Receptor Mediates Binding and Cytotoxicity of Plant Ribosome‐Inactivating Proteins

Cavallaro, Ugo; Nykjaer, Anders; Nielsen, Morten S.; Soria, Marco R.

doi:10.1111/j.1432-1033.1995.tb20795.x

Cited by 60 publications

(49 citation statements)

References 61 publications

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“…In addition, SAP-C also bound equally well to α2MR (Table 3). Binding could be inhibited by EDTA, heparin and both the competitors LpL and RAP, as previously shown for SAP-S [31]. This confirms the specificity of α2MR binding (Table 3).…”

Section: Ribosome-inactivating Activity Of Recombinant Saporin Isoformssupporting

confidence: 87%

“…Most of these studies have been carried out on the internalization pathway of the ricin holotoxin [30]. We previously demonstrated that saporin entry into the cells is not a passive mechanism as was generally believed, but is mediated by a large and widespread receptor, the α2MR [31]. α2MR is a multifunctional endocytic receptor bearing multiple binding sites [32].…”

Section: Ribosome-inactivating Activity Of Recombinant Saporin Isoformsmentioning

confidence: 99%

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Characterization of a saporin isoform with lower ribosome-inhibiting activity

Fabbrini

Rappocciolo

Carpani

et al. 1997

Biochemical Journal

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We have expressed in Escherichia coli five isoforms of saporin, a single-chain ribosome-inactivating protein (RIP). Translation inhibition activities of the purified recombinant polypeptides in itro were compared with those of recombinant dianthin 30, a less potent and closely related RIP, and of ricin A chain. Dianthin 30, and a saporin isoform encoded by a cDNA from leaf tissue (SAP-C), both had about one order of magnitude lower activity in translation inhibition assays than all other isoforms of saporin tested. We recently demonstrated that saporin extracted from seeds of Saponaria officinalis binds to α2-macroglobulin receptor (α2MR ; also termed low density lipoprotein-receptor-related-protein), indicating a general mechanism of interaction of plant RIPs with the α2MR system [Cavallaro, Nykjaer, Nielsen and Soria (1995) Eur. J. Biochem.

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Section: Ribosome-inactivating Activity Of Recombinant Saporin Isoformssupporting

confidence: 87%

Section: Ribosome-inactivating Activity Of Recombinant Saporin Isoformsmentioning

confidence: 99%

Characterization of a saporin isoform with lower ribosome-inhibiting activity

Fabbrini

Rappocciolo

Carpani

et al. 1997

Biochemical Journal

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“…RTA has a very low lysine content and a slightly acidic pI whereas 10% of the amino acids in SAP are lysine residues, which confer also an extremely high pI (almost 10) to this polypeptide. In addition, SAP can be internalized through members of the low-density lipoprotein-related receptor family 15,16 and has a much higher cell-free RIP activity, compared to RTA. 15,16 Acting catalytically, SAP has very high intrinsic activity as it has been established that only a few molecules of toxin reaching the cytosolic compartment are sufficient to inhibit protein synthesis and cause cell death.…”

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confidence: 99%

“…In addition, SAP can be internalized through members of the low-density lipoprotein-related receptor family 15,16 and has a much higher cell-free RIP activity, compared to RTA. 15,16 Acting catalytically, SAP has very high intrinsic activity as it has been established that only a few molecules of toxin reaching the cytosolic compartment are sufficient to inhibit protein synthesis and cause cell death. 17 Seed-extracted SAP has been widely used to develop mouse models selectively impaired in central nervous system functions.…”

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Saporin as a novel suicide gene in anticancer gene therapy

et al. 2006

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We used a non-viral gene delivery approach to explore the potential of the plant saporin (SAP) gene as an alternative to the currently employed suicide genes in cancer therapy. Plasmids expressing cytosolic SAP were generated by placing the region encoding the mature plant ribosome-inactivating protein under the control of cytomegalovirus (CMV) or simian virus 40 (SV40) promoters. Their ability to inhibit protein synthesis was first tested in cultured tumor cells co-transfected with a luciferase reporter gene. In particular, SAP expression driven by CMV promoter (pCI-SAP) demonstrated that only 10 ng of plasmid per 1.6 Â 10 4 B16 cells drastically reduced luciferase activity to 18% of that in control cells. Direct intratumoral injection of pCI-SAP complexed with either lipofectamine or N-(2,3-dioleoyloxy-1-propyl) trimethylammonium methyl sulfate (DOTAP) in B16 melanoma-bearing mice resulted in a noteworthy attenuation of tumor growth. This antitumor effect was increased in mice that received repeated intratumoral injections. A SAP catalytic inactive mutant (SAP-KQ) failed to exert any antitumor effect demonstrating that this was specifically owing to the SAP N-glycosidase activity. Our overall data strongly suggest that the gene encoding SAP, owing to its rapid and effective action and its independence from the proliferative state of target cells might become a suitable candidate suicide gene for oncologic applications.

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“…More recent results analyzed in 0.8% agarose and/or in 6% polyacrylamide gel electroobtained by others also suggest a possible penetration of the phoresis. DNA bands were visualized by staining with ethidium brosc-RIPs into cells [12,13]. In the light of our results and of mide [17].…”

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confidence: 85%

DNA‐nuclease activity of the single‐chain ribosome‐inactivating proteins dianthin 30, saporin 6 and gelonin

Roncuzzi

Gasperi‐Campani

1996

FEBS Letters

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The single-chain ribosome-inactivating proteins (scRIPs) The so-RIPs asparin 1, dianthin 30, gelonin, momordin, PAP-S identified and mapped in pBR322.(pokeweed antiviral protein from Phytolacca americana seeds) and saporin 6 were highly purified as described previously [15]. HPLCpurified saporin 6, whose specific N-glycosidase activity had been Agarose and acrylamide/bis-acrylamide for gel electrophoresis were to the A-chains of ricin and related toxins [2], which are purchased from Clontech Laboratories, Palo Alto, CA (USA). All known to depurinate the ribosomal RNA by cleaving the Nother chemicals were of analytical grade.glycosidic bond in the A4324 position of the 28S RNA fracRestriction nucleases employed were: PvuII (from Proteus vulgaris) tion, so rendering it incapable of binding to the elongation incubation buffer: Tris-HCl 10 raM, NaC1 100 mM, MgCI2 10 mM, factors, with the consequent arrest of protein synthesis [3,4]. dithioerythritol 1 mM, pH 7.5 at 37°C; PstI (from Providencia stuartii) and HinfI (from Haemophylus influenzae Rf) incubation buffer: These proteins have attracted interest in the construction of Tris-HC1 50 mM, NaCI 10 raM, MgCI2 10 mM, dithioerythritol 1 immunotoxins after conjugation with monoclonal antibodies raM, pH 7.5 at 37°C; BamHI (from Bacillus amyloliquefacens H) for the selective killing of neoplastic cells [5 7].and HindIII (from Haemophylus influenzae Rd com-10) incubation To better understand perspectives and limits of the sc-RIPs buffer: Tris-HC1 10 mM, NaC1 100 raM, MgCI2 5 mM, 2-mercaptoethanol 1 mM, pH 8 at 37°C. in clinical trials, we previously focused our attention on the antiproliferative effect of RIPs as native molecules or in corn-2.2. DNase activity assay bination with other drugs. We have demonstrated that the pBR322 and OX174 plasmid DNA (250 ng), single-stranded M13 native form of the sc-RIP saporin 6 exerts an antiproliferative phage, lambda phage DNA, linearized plasmid DNA (250 ng) were incubated with or without various amounts (250-0.25 ng) of the dieffect in vitro in human breast cancer, leukemia and melanoverse proteins in a final volume of 10 ~tl at 37°C for various times. The ma cells to a very different extent and with diverse kinetics, reactions were carried out in a range of 5 60 mM NaC1 (or MgC12), l dependent on the specific cell target analyzed [8][9][10]. The efmM Tris-HC1, 0.1 mM EDTA. The range of pH was 6.5-8. At the fect may be potentiated by other drugs: a strong synergism end of the incubations, all the samples were extracted with phenol has been obtained by combination of saporin 6 with lonidfollowed by ether and precipitated [17]. Digestion with restriction endonucleases was carried out as specified above. The samples were amine in breast cancer cells in vitro [11]. More recent results analyzed in 0.8% agarose and/or in 6% polyacrylamide gel electroobtained by others also suggest a possible penetration of the phoresis. DNA bands were visualized by staining with ethidium brosc-RIPs into cells [12,13]. In the light of our resu...

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α₂‐Macroglobulin Receptor Mediates Binding and Cytotoxicity of Plant Ribosome‐Inactivating Proteins

Cited by 60 publications

References 61 publications

Characterization of a saporin isoform with lower ribosome-inhibiting activity

Characterization of a saporin isoform with lower ribosome-inhibiting activity

Saporin as a novel suicide gene in anticancer gene therapy

DNA‐nuclease activity of the single‐chain ribosome‐inactivating proteins dianthin 30, saporin 6 and gelonin

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α2‐Macroglobulin Receptor Mediates Binding and Cytotoxicity of Plant Ribosome‐Inactivating Proteins

Cited by 60 publications

References 61 publications

Characterization of a saporin isoform with lower ribosome-inhibiting activity

Characterization of a saporin isoform with lower ribosome-inhibiting activity

Saporin as a novel suicide gene in anticancer gene therapy

DNA‐nuclease activity of the single‐chain ribosome‐inactivating proteins dianthin 30, saporin 6 and gelonin

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α₂‐Macroglobulin Receptor Mediates Binding and Cytotoxicity of Plant Ribosome‐Inactivating Proteins