Add to ORKGA method of assembly of a single-chain Fv fragment is described, whereby asymmetric polymerase chain reactions (APCR) and primer extension were used to join immunoglobulin heavy and light chain variable region genes via a linker sequence. In this procedure heavy and light chain genes, together with a linker gene containing complementary sequences, were amplified by APCR to generate single-stranded products. The single stranded heavy or light chain genes were hybridized to the relevant single-stranded link product, and extended to produce double-stranded heavy-link and link-light genes. These genes then underwent another round of APCR, resulting in two single-stranded genes (heavy-link and link-light) containing extensive overlapping sequenc...
We have mimicked features of immune selection to make human antibodies in bacteria. Diverse librarie...
A rapid route for the generation of monoclonal antibodies by repertoire cloning is described. The te...
The use of a recombinant antibody fragment instead of a complete antibody, as a conformational probe...
Cloning the correct VL kappa gene from hybridomas derived from MOPC-21 can be problematic because su...
This chapter discusses the expression and genetic manipulation of antibody fragments in E. coli. The...
We describe a general approach to rapidly obtain the DNA sequence encoding the variable region of an...
We have devised a strategy based on polymerase chain reaction (PCR) for the rapid cloning of functio...
In this chapter, protocols are described for converting mouse monoclonal antibodies into recombinant...
We describe a new method for amplification, by polymerase chain reaction (PCR), of rearranged segmen...
A number of recent technological developments have greatly facilitated the genetic engineering of im...
Monoclonal antibodies are produced in cultured hybridoma cell lines, but these cells tend to be unst...
A new plasmid vector, pCRP, allowing the expression of human recombinant monoclonal antibody Fab fra...
Effects of nucleotide sequences of polypeplide linkers on production of soluble single-chain Fv anti...
We constructed a single-chain Fv antibody library that permits human complementarity-determining reg...
The hypervariable loops of an antibody molecule are supported on the relatively conserved β-sheeted ...
We have mimicked features of immune selection to make human antibodies in bacteria. Diverse librarie...
A rapid route for the generation of monoclonal antibodies by repertoire cloning is described. The te...
The use of a recombinant antibody fragment instead of a complete antibody, as a conformational probe...
Cloning the correct VL kappa gene from hybridomas derived from MOPC-21 can be problematic because su...
This chapter discusses the expression and genetic manipulation of antibody fragments in E. coli. The...
We describe a general approach to rapidly obtain the DNA sequence encoding the variable region of an...
We have devised a strategy based on polymerase chain reaction (PCR) for the rapid cloning of functio...
In this chapter, protocols are described for converting mouse monoclonal antibodies into recombinant...
We describe a new method for amplification, by polymerase chain reaction (PCR), of rearranged segmen...
A number of recent technological developments have greatly facilitated the genetic engineering of im...
Monoclonal antibodies are produced in cultured hybridoma cell lines, but these cells tend to be unst...
A new plasmid vector, pCRP, allowing the expression of human recombinant monoclonal antibody Fab fra...
Effects of nucleotide sequences of polypeplide linkers on production of soluble single-chain Fv anti...
We constructed a single-chain Fv antibody library that permits human complementarity-determining reg...
The hypervariable loops of an antibody molecule are supported on the relatively conserved β-sheeted ...
We have mimicked features of immune selection to make human antibodies in bacteria. Diverse librarie...
A rapid route for the generation of monoclonal antibodies by repertoire cloning is described. The te...
The use of a recombinant antibody fragment instead of a complete antibody, as a conformational probe...