Chimeric Ecotropic MLV Envelope Proteins that Carry EGF Receptor-Specific Ligands and the Pseudomonas Exotoxin A Translocation Domain to Target Gene Transfer to Human Cancer Cells

Erlwein, Otto; Wels, Winfried S.; Schnierle, Barbara S.

doi:10.1006/viro.2002.1517

Cited by 13 publications

(12 citation statements)

References 35 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Attempts to change the tropism of a virus by engineering its RBD, either by insertion of ligands to known cell surface proteins (16,19,20,27,37) or by selection of randomized libraries (11), have had various degrees of success. Common to all of the previously engineered viral envelopes is that none of them was as efficient as the wild-type envelope.…”

Section: Discussionmentioning

confidence: 99%

Change of Tropism of SL3-2 Murine Leukemia Virus, Using Random Mutational Libraries

Bahrami

Duch²,

Pedersen

2004

J Virol

View full text Add to dashboard Cite

SL3-2 is a polytropic murine leukemia virus with a limited species tropism. We cloned the envelope gene of this virus, inserted it into a bicistronic vector, and found that the envelope protein differs from other, similar envelope proteins that also utilize the polytropic receptor (Xpr1) in that it is severely impaired in mediating infection of human and mink cells. We found that two adjacent amino acid mutations (G212R and I213T), located in a previously functionally uncharacterized segment of the surface subunit, are responsible for the restricted tropism of the SL3-2 wild-type envelope. By selection from a two-codon library, several hydrophobic amino acids at these positions were found to enable the SL3-2 envelope to infect human TE 671 cells. In particular, an M212/V213 mutant had a titer at least 6 orders of magnitude higher than that of the wild-type envelope for human TE 671 cells and infected human, mink, and murine cells with equal efficiencies. Notably, these two amino acids are not found at homologous positions in known murine leukemia virus isolates. Functional analysis and library selection were done on the basis of sequence and tropism analyses of the SL3-2 envelope gene. Similar approaches may be valuable in the design and optimization of retroviral envelopes with altered tropisms for biotechnological purposes.The murine leukemia virus (MLV) group of gammaretroviruses has been divided into the ecotropic, amphotropic, and polytropic-xenotropic subfamilies according to their host range and interference properties, as determined primarily on the basis of the structures of their respective envelope glycoproteins.The envelope precursor protein is cleaved into two subunits in the endoplasmic reticulum by a cellular protease. The Nterminal surface subunit (SU) is mainly responsible for receptor recognition and binding, while the C-terminal transmembrane subunit is involved in the fusion of the viral and cellular membranes. Accordingly, the SU subunits of different MLV subfamilies show a considerable degree of residue disparity, especially in the N-terminal 200 to 250 residues, while the transmembrane subunits are very much identical. Interestingly, the N terminus of the SU subunit constitutes a receptor-binding domain (RBD), which can bind to the appropriate receptor independently of the rest of the envelope protein. Thus, the ecotropic RBD, which consists of the first 230 (4) or 245 (22) residues, contains almost all of the unique ecotropic envelope sequences. This domain is followed by a proline-rich region that can tolerate large insertions or deletions (15,36).Three segments of the RBD that show large variations in MLV subfamilies are conveniently known as hypervariable regions A, B, and C (VRA, VRB, and VRC, respectively). Several studies have suggested that the determinants of the tropisms of ecotropic and amphotropic envelopes are found in the N terminus of RBD, particularly VRA, while segments further downstream are partially responsible for polytropic envelope tropism (4,7,8,25,29).Ecotropic and...

show abstract

Section: Discussionmentioning

confidence: 99%

Change of Tropism of SL3-2 Murine Leukemia Virus, Using Random Mutational Libraries

Bahrami

Duch²,

Pedersen

2004

J Virol

View full text Add to dashboard Cite

show abstract

“…We inserted GFP at the N terminus and into the proline-rich region (PRR) of Env ( Fig. 1A) because these regions have been shown to tolerate large insertions (Cosset et al, 1995;Kayman et al, 1999;Wu et al, 2000;Erlwein et al, 2002). For insertion into the PRR, the enhanced GFP sequences of plasmid pSFG-EGFP (Lindemann et al, 1997) were amplified by PCR using the primers 59EGFP (59-AAAACC ACCCAGTGGGGTGAGCAAGGGCGAGGAGCTG-39) and 39EGFP (59-AAAACGCCGGTGGACTTGTACAGCTCGT CCATGC-39); GFP sequences are indicated in bold.…”

mentioning

confidence: 99%

“…For insertion into the PRR, the enhanced GFP sequences of plasmid pSFG-EGFP (Lindemann et al, 1997) were amplified by PCR using the primers 59EGFP (59-AAAACC ACCCAGTGGGGTGAGCAAGGGCGAGGAGCTG-39) and 39EGFP (59-AAAACGCCGGTGGACTTGTACAGCTCGT CCATGC-39); GFP sequences are indicated in bold. The amplicon was then inserted between the PflMI and SgrAI sites of pwt(HX), an expression plasmid for MoMLV Env (Erlwein et al, 2002). In addition, a unique SnaBI site was engineered for future cloning purposes behind the regenerated SgrAI site by inserting the oligonucleotides 59SNA (59-CCGGTGCGTACGTA-39) and 39SNA (59-CCGGTACGTACGCA-39).…”

mentioning

confidence: 99%

The proline-rich region of the ecotropic Moloney murine leukaemia virus envelope protein tolerates the insertion of the green fluorescent protein and allows the generation of replication-competent virus

Erlwein

Buchholz

Schnierle

2003

Journal of General Virology

Self Cite

View full text Add to dashboard Cite

Sequences encoding the green fluorescent protein (GFP) were inserted into the envelope protein (Env) of ecotropic Moloney murine leukaemia virus, MoMLV. Insertion of these sequences into the proline-rich region (PRR) of Env resulted in a chimeric GFP-Env protein that allowed retrovirus vector transduction of murine cells with titres similar to wild-type Env. However, N-terminal extension with GFP did not result in a functional Env protein. GFP sequences were then inserted into the Env PRR of E-MO virus, a MoMLV that carries epidermal growth factor sequences at the N terminus of its Env protein. The resulting virus, GFP-EMO1, replicates to the same titres as the parental virus. In a chronically infected cell culture, GFP-EMO1 was genetically stable. However, additional insertions of sequences that led to recombination or that may have been incompatible with virus replication were deleted and decreased virus titre. In summary, Env PRR can be used to tag individual virus particles with GFP, which leaves other regions available for modification in studies aimed at altering virus tropism.The processes that are involved in adsorption and internalization of retroviruses are not fully understood. To visualize entry of a virus into the cell, we constructed a modified ecotropic Moloney murine leukaemia virus (MoMLV) bearing the green fluorescent protein (GFP) from Aequoria victoria in its envelope (Env). We inserted GFP at the N terminus and into the proline-rich region (PRR) of Env (Fig. 1A) because these regions have been shown to tolerate large insertions (Cosset et al., 1995;Kayman et al., 1999;Wu et al., 2000;Erlwein et al., 2002). For insertion into the PRR, the enhanced GFP sequences of plasmid pSFG-EGFP (Lindemann et al., 1997) were amplified by PCR using the primers 59EGFP (59-AAAACC ACCCAGTGGGGTGAGCAAGGGCGAGGAGCTG-39) and 39EGFP (59-AAAACGCCGGTGGACTTGTACAGCTCGT CCATGC-39); GFP sequences are indicated in bold. The amplicon was then inserted between the PflMI and SgrAI sites of pwt(HX), an expression plasmid for MoMLV Env (Erlwein et al., 2002). In addition, a unique SnaBI site was engineered for future cloning purposes behind the regenerated SgrAI site by inserting the oligonucleotides 59SNA (59-CCGGTGCGTACGTA-39) and 39SNA (59-CCGGTACGTACGCA-39). In the resulting protein, GFP-Env1, GFP sequences replaced the amino acids between positions 265 and 273 of Env. In GFP-Env2, GFP sequences were inserted between amino acids 6 and 7 of Env. Humanized GFP (S 65 RT mutant) sequences were excised from plasmid pCMV-hGFP (Clontech) and inserted inframe into the HindIII/XhoI site of pSG-env . Constructs are delineated in Fig. 1(A).After transient transfection, cells expressing GFP-Env1 or GFP-Env2 showed fluorescence, demonstrating the functionality of the GFP sequences in the Env environment. We then carried out transduction experiments to see whether the presence of GFP sequences affected virus titre. The packaging cell line Anjou 65 produces the structural proteins Gag and Pol (Pear et al., 1993). Upon transfection with a ...

show abstract

“…Ecotropic envelopes have generally been used as experimental systems for retargeting efforts since their limited tropism (capable of infecting only murine cells) makes them adaptable to such experiments. However, most attempts to produce an envelope protein capable of utilizing a heterologous protein as entry receptor either have been unsuccessful or have resulted in tropism change with severely reduced infection efficiencies (5,13,17,21,31). Only in two cases has efficient retargeting been achieved.…”

Section: Discussionmentioning

confidence: 99%

“…Several attempts to retarget ecotropic MLV through insertion of single-chain antibodies into SU have failed mainly because the resulting envelopes cannot induce the fusion of membranes after binding to the new receptors. In other cases, insertion of peptide ligands into SU has been used to confer new tropism, usually resulting in very inefficient retargeted envelope proteins (5,13,17,21,31). However, two cases of efficient targeting have been reported, both based on ecotropic MLVs.…”

mentioning

confidence: 99%

Construction of a Gammaretrovirus with a Novel Tropism and Wild-Type Replication Kinetics Capable of Using Human APJ as Entry Receptor

Bahrami

Pagh

Ejegod

et al. 2012

J Virol

View full text Add to dashboard Cite

We have constructed a replication-competent gammaretrovirus (SL3-AP) capable of using the human G-protein-coupled receptor hAPJ as its entry receptor. The envelope protein of the virus was made by insertion of the 13-amino-acid peptide ligand for hAPJ, flanked by linker sequences, into one of the variable loops of the receptor binding domain of SL3-2, a murine leukemia virus (MLV) that uses the xenotropic-polytropic virus receptor Xpr1 and which has a host range limited to murine cells. This envelope protein can utilize hAPJ as well as murine Xpr1 for entry into host cells with equal efficiencies. In addition, the SL3-AP virus replicates in cells expressing either of its receptors, hAPJ and murine Xpr1, and causes resistance to superinfection and downregulation of hAPJ in infected cells. Thus, SL3-AP is the first example of a retargeted replication-competent retrovirus, with replication characteristics and receptor interference properties similar to those of natural isolates.

show abstract

Chimeric Ecotropic MLV Envelope Proteins that Carry EGF Receptor-Specific Ligands and the Pseudomonas Exotoxin A Translocation Domain to Target Gene Transfer to Human Cancer Cells

Cited by 13 publications

References 35 publications

Change of Tropism of SL3-2 Murine Leukemia Virus, Using Random Mutational Libraries

Change of Tropism of SL3-2 Murine Leukemia Virus, Using Random Mutational Libraries

The proline-rich region of the ecotropic Moloney murine leukaemia virus envelope protein tolerates the insertion of the green fluorescent protein and allows the generation of replication-competent virus

Construction of a Gammaretrovirus with a Novel Tropism and Wild-Type Replication Kinetics Capable of Using Human APJ as Entry Receptor

Contact Info

Product

Resources

About