Selection of feline leukemia virus envelope proteins from a library by functional association with a murine leukemia virus envelope

Bupp, Keith; Sarangi, Anindita; Roth, Monica J.

doi:10.1016/j.virol.2006.03.040

Cited by 11 publications

(17 citation statements)

References 41 publications

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“…The introduction of plasmid CeB (46) expressing the gag-pol gene into human TE671 cells producing TECeB [F2 isolate; (47)] and TELCeB6 cells expressing the ⌿ ϩ lacZ gene plus CeB (46) were previously described. The maintenance of the human DU145, human A498, human TE671, TECeB, TELCeB6 cells, human 293T, 293TCeB, and feline AH927 were as previously described (21,22).…”

Section: Methodsmentioning

confidence: 99%

Identification of a retroviral receptor used by an Envelope protein derived by peptide library screening

Sarangi¹,

Bupp²,

Roth³

2007

Proc. Natl. Acad. Sci. U.S.A.

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(11)(12)(13)] viral receptors. With these evolutionary observations, it is of great interest as to whether a given retrovirus must remain restricted to use receptors within the broad class of the original receptor or can be altered to use receptors beyond these protein family boundaries.A variety of approaches have been developed for altering the receptor usage of viral delivery systems. Receptor specificity and binding of the viral Envelope (Env) is mapped to the N-terminal half of the surface (SU) protein through the close interaction of two highly variable regions, VR1 (VRA) and VR2 (VRB) (14-18). Exchange of a defined VR1 segment between the FeLV A and C subgroups altered the viral host range (19). In our studies, codons for 10/11 amino acids within this VR1 FeLV Env receptor-binding region were randomized within a FeLV A/C Env chimera backbone (20). Viral particles bearing this library of Ͼ1 million viral VR1 Env variants are selected for productive infection (20)(21)(22). This library displays the targeting peptide within the context of the authentic Env backbone, eliminating the problem that preidentified phage display peptides inserted into alternative contexts do not maintain their original properties (23). Alternative approaches have involved the addition of targeting domains (24, 25), peptides (23, 26), or single-chain antibodies (27) within the framework of viral Env or capsids (28-30) or through heterologous intermediates (31). Successful retargeting for Sindbis Env pseudotyped onto lentiviral particles has been achieved with the insertion of the Protein A ZZ domain and sandwiching targeting antibodies to the modified particles (32) or through coexpression of Env proteins and surfacebinding molecules (33).Screening the FeLV random Env library on feline AH927 cells identified the A5 Env isolate, which also efficiently infected human 293T embryonic kidney cells (21). Superinfection interference studies indicated that the receptor for A5 was outside the receptor family used by FeLV A, B, and C and MuLV 4070A viruses (21). The A5 Env therefore provided an excellent system to examine the range of proteins capable of serving as receptors for retroviral Env libraries. In this study, the receptor for the A5 Env isolate was identified as the SLC35F2 protein, a transporter protein of unknown function, through screening a feline AH927 cDNA library. ResultsDirected evolution allows for the selection of proteins with new properties. Using this approach, randomization of the FeLV Env receptor-binding domain, followed by selection for productive infection, identified Env isolates with receptor usage outside the interference groups of the known FeLV A, B, and C viruses (21,22). This result implies that the selection of a receptor protein can occur through screening a single round of viral infection. To definitively prove that alternative viral receptors can be selected, the receptor protein for the A5 Env isolate was identified through cDNA screening. The authors declare no conflict of interest.Abbreviations: Env,...

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Section: Methodsmentioning

confidence: 99%

Identification of a retroviral receptor used by an Envelope protein derived by peptide library screening

Sarangi¹,

Bupp²,

Roth³

2007

Proc. Natl. Acad. Sci. U.S.A.

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“…Large pools of viral envelope mutants can be generated using a number of approaches, including randomly shuffling gene templates from different parent viruses , inserting random peptide sequences at a specific location Roth, 2002, 2003;Bupp et al, 2005Bupp et al, , 2006, or inserting a defined peptide into random locations Schaffer, 2006a, 2006b). The resulting envelope mutant genetic library is inserted into recombinant viral genomes, and each envelope protein mutant is packaged to generate virus particles encompassing the genome that encodes it.…”

Section: Retroviral Vectorsmentioning

confidence: 99%

“…Some of the earliest efforts to apply library selection approaches to target retroviral vectors involved libraries where short, random peptide sequences were genetically substituted into the receptor-determining region (RDR) of feline leukemia virus subgroup A (FeLV-A) envelope proteins followed by selection on target cells (Table I) Roth, 2002, 2003;Bupp et al, 2005Bupp et al, , 2006. In contrast to MLV envelope proteins that require changes in both variable regions of their receptor-binding domain (VRA and VRB), modification of only the VRA domains of FeLV envelope proteins allows modulation of viral tropism without severe structural perturbation (Bupp and Roth, 2002).…”

Section: Cell Receptor-specific or Transductional Targetingmentioning

confidence: 99%

“…Furthermore, a library, whose individual viral particle variants contained/displayed both the same random peptide library as well as amphotropic murine leukemia 4070A virus envelope proteins on their surfaces, yielded an interesting result after selection on 4070A-infected PC-3 human prostate cells. The envelope protein variants that emerged from this selection apparently cooperated with 4070A envelope proteins to infect PC-3 cells, such that preinfection of these cells with wild-type 4070A retrovirus prior to addition of the novel viruses competed away most but not all of the latter's infectivity (Bupp et al, 2006). Both rational ligand insertion and random peptide display require knowledge of insertion sites that do not compromise envelope function and are exposed on the protein surface for receptor binding Roth, 2002, 2003;Bupp et al, 2005Bupp et al, , 2006.…”

Section: Cell Receptor-specific or Transductional Targetingmentioning

confidence: 99%

“…The envelope protein variants that emerged from this selection apparently cooperated with 4070A envelope proteins to infect PC-3 cells, such that preinfection of these cells with wild-type 4070A retrovirus prior to addition of the novel viruses competed away most but not all of the latter's infectivity (Bupp et al, 2006). Both rational ligand insertion and random peptide display require knowledge of insertion sites that do not compromise envelope function and are exposed on the protein surface for receptor binding Roth, 2002, 2003;Bupp et al, 2005Bupp et al, , 2006. However, if information on such permissive insertion sites is not available, it can be also newly obtained by transposon-based scanning of envelope proteins (Rothenberg et al, 2001;Yu and Schaffer, 2006b).…”

Section: Cell Receptor-specific or Transductional Targetingmentioning

confidence: 99%

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Library selection and directed evolution approaches to engineering targeted viral vectors

Jang

Lim

Schaffer

2007

Biotech & Bioengineering

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Gene therapy, to delivery of genetic material to a patient for therapeutic benefit, has significant promise for translating basic knowledge of disease mechanism into biomedical treatments. The clinical development of the field has been slowed, however, by the need for improvements in the properties and capabilities of gene delivery vehicles. Vehicles based on viruses offer the potential for efficient gene delivery, but because viruses did not evolve to serve human therapeutic needs, many of their properties require significant improvement, including their safety, efficiency, and capacity for targeted gene delivery. Since viruses are highly complex biological entities, engineering such properties at the molecular level can be challenging. However, there has been significant progress in developing approaches that mimic the mechanisms by which viruses arose in the first place. In particular, library-based selection, the generation of one diverse genetic library and selection for new properties, and directed evolution, based on the multiple rounds of library generation and selection for iterative improvement of function, have strong potential in engineering novel properties into these complex biomolecular assemblies. This review will discuss progress in the application of peptide display, library selection, and directed evolution technologies toward engineering vectors based on retrovirus, adeno-associated virus, and adenovirus that are capable of targeted delivery to specific cell types. In addition to creating biomedically useful products, these approaches have future potential to yield novel insights into viral structure-function relationships.

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Designer Gene Delivery Vectors: Molecular Engineering and Evolution of Adeno-Associated Viral Vectors for Enhanced Gene Transfer

2007

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Abstract. Gene delivery vectors based on adeno-associated virus (AAV) are highly promising due to several desirable features of this parent virus, including a lack of pathogenicity, efficient infection of dividing and non-dividing cells, and sustained maintenance of the viral genome. However, several problems should be addressed to enhance the utility of AAV vectors, particularly those based on AAV2, the best characterized AAV serotype. First, altering viral tropism would be advantageous for broadening its utility in various tissue or cell types. In response to this need, vector pseudotyping, mosaic capsids, and targeting ligand insertion into the capsid have shown promise for altering AAV specificity. In addition, library selection and directed evolution have recently emerged as promising approaches to modulate AAV tropism despite limited knowledge of viral structure-function relationships. Second, preexisting immunity to AAV must be addressed for successful clinical application of AAV vectors. BShielding^polymers, site-directed mutagenesis, and alternative AAV serotypes have shown success in avoiding immune neutralization. Furthermore, directed evolution of the AAV capsid is a high throughput approach that has yielded vectors with substantial resistance to neutralizing antibodies. Molecular engineering and directed evolution of AAV vectors therefore offer promise for generating Fdesigner_ gene delivery vectors with enhanced properties.

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Selection of feline leukemia virus envelope proteins from a library by functional association with a murine leukemia virus envelope

Cited by 11 publications

References 41 publications

Identification of a retroviral receptor used by an Envelope protein derived by peptide library screening

Identification of a retroviral receptor used by an Envelope protein derived by peptide library screening

Library selection and directed evolution approaches to engineering targeted viral vectors

Designer Gene Delivery Vectors: Molecular Engineering and Evolution of Adeno-Associated Viral Vectors for Enhanced Gene Transfer

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