1 Biochemisches Institut der Universität Zürich, Winterthurerstrasse 190,CH-8057 Zürich, Switzerland and 2 Industrial Biochemistry Group, Department of Chemical and Environmental Sciences, University of Limerick, Limerick, Ireland
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Abstract |
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Keywords: antibody engineering /protein folding/protein misfolding/protein aggregation/rational design
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Introduction |
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Recombinant antibody fragments require disulfide bonds for activity and this necessitates their secretion into the bacterial periplasm in order to come in contact with the disulfide forming machinery (Bardwell, 1994). While disulfide formation is possible in the cytoplasm in special strains (Derman et al., 1993
; Proba et al., 1995
), the oxidation is generally inefficient. In the periplasm, native Fv, Fab or single-chain Fv (scFv) fragments can be obtained with correct domain association (Plückthun et al., 1996
). The limiting step in this process is frequently that of periplasmic folding, with some proteins following an aggregation reaction that competes with the correct folding pathway in vivo. While this periplasmic expression approach has been successfully used in the production of many recombinant antibody fragments, the efficiency of folding has been shown to be strongly dependent upon the protein which is being produced (Knappik and Plückthun, 1995
; Ullrich et al., 1995
; Forsberg et al., 1997
; Jung and Plückthun, 1997
; Nieba et al., 1997
).
A previous study of the folding of the anti-phosphorylcholine (PC) antibody McPC603 identified a number of heavy chain framework mutations in this antibody that increase the yield of correctly folded, functional fragments in E.coli (Knappik and Plückthun, 1995). The phosphorylcholine response in the BALB/c mouse is characterized by a restricted usage of gene segments (Perlmutter et al., 1984
; Malipiero et al., 1987
). The VH gene used is called VT15 since the antibody TEPC15 (or T15), originally found as a myeloma IgA, carries the unaltered sequence. The well characterized myeloma antibodies McPC603 (or M603) and MOPC167 (or M167) also use the same V, D and J segments in the heavy chain, but carry different somatic mutations, and N-region diversity and some truncation lead to rather different CDR-H3 loops (Perlmutter et al., 1984
; Malipiero et al., 1987
; Plückthun, 1993
). All three antibodies have different light chains, derived from V
8 (M603), V
24 (M167) and V
32 (T15). The crystal structures of the Fab fragment of M603 (Satow et al., 1986
) and the recombinant VL domain (Steipe et al., 1992
) have been determined, and the Fv and scFv fragments have been studied by NMR (Freund et al., 1994
).
We describe here the results of our investigation of the folding of antibody domains in E.coli, using the anti-PC antibody T15. The T15 antibody was chosen for this study as it has been found in the past to be produced at very low levels in E.coli, to be produced in a non-functional form, and to be highly susceptible to proteolytic degradation (Plückthun and Pfitzinger, 1991), yet to be closely related to the more efficiently expressed McPC603. Because of their close sequence similarity we could pinpoint factors limiting the folding of T15 and the hierarchy of mutational effects. We report our studies on a systematic investigation of this model antibody, resulting in the generation of stable, functional T15 antibody fragments.
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Materials and methods |
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The bacterial strain used throughout this study was E.coli JM83 [ara (lac-proAB), rpsL (strA), thi, [
80 dlacZ
M15] (Yanisch-Perron et al., 1985
)]. The anti-PC antibodies were expressed as Fv and single-chain Fv (scFv) fragments from the pHJ300 series of vectors (Knappik and Plückthun, 1995
; Ge et al., 1995
).
Expression of antibody fragments
Bacteria harbouring the relevant pHJ300 vector were grown overnight, with shaking, at 37°C in 5 ml LB medium containing streptomycin (25 µg/ml) and ampicillin (100 µg/ml). A 25 ml volume of this culture, depending on the OD550, was pelleted by centrifugation and resuspended in 0.5 ml LB. This cell washing was repeated once in order to reduce carry-over of ß-lactamase that might break down ampicillin and facilitate the growth of plasmid-free cells. The resuspended cells were then added to 19.5 ml LB containing ampicillin and streptomycin as above and shaken in a water bath at 24°C until an OD of 0.5 was reached. Induction of antibody fragment production was achieved by the addition of 1 mM IPTG (final concentration). At the time of induction and for every hour thereafter, 200 µl samples of culture were removed; of this, 100 µl was used to determine the OD550 of the culture and the remainder to measure the ß-lactamase activity in the culture supernatant, according to O'Callaghan and co-workers (1972). As the exact shape of each growth curve can be affected by many environmental parameters, each growth experiment was carried out three times on different days, with all mutants of interest assessed in parallel.
Protein production and analysis
Following harvesting of induced cultures, soluble and insoluble protein fractions were separated as previously described (Knappik and Plückthun, 1995). SDSPAGE and immunoblotting were carried out using standard procedures and bacterially produced antibody fragments were detected using the commercially available M1 antibody (Prickett et al., 1989
; Knappik and Plückthun, 1994
), directed against the 4-amino acid FLAG peptide encoded at the N-terminal end of the fragments.
Mutagenesis of the antibody fragments
Introduction of the previously-described framework H40, H60 and H61 mutations (Kabat numbering), collectively termed the `H11 mutations' (Knappik and Plückthun, 1995), into the T15 fragments was carried out according to Kunkel and co-workers (1987). Clones into which the mutations had been introduced were confirmed by Sanger dideoxy sequencing. Mutated clones were sequenced between convenient restriction sites in the vector and the mutated DNA was cloned back into the original expression vector for protein production and analysis. Exchange of CDRs between the three antibodies was carried out by restriction digestion cloning. Site-directed mutagenesis of the VL domain was achieved using the splicing by overlap extension method (SOE) of Ho and co-workers (1989).
Affinity chromatography
Protein production for affinity chromatography was carried out essentially as described by Knappik and Plückthun (1995). An overnight culture in 10 ml SB medium (20 g/l tryptone, 10 g/l yeast extract, 5 g/l NaCl, 2.5 g/l K2HPO4, 1 g/l Mg2SO4.7H2O) containing streptomycin (25 µg/ml) and ampicillin (100 µg/ml) was used to inoculate 2 l of the same medium in a 5 l culture flask. Cultures were shaken at 24°C until an OD550 of 0.5 was reached and were then induced by the addition of IPTG to a concentration of 1 mM. Induction was allowed to continue until shortly before extensive periplasmic leakiness began to occur, as determined from the smaller scale growth experiments described above. In the case of most clones studied, this involved a 3 h induction period. Cells were then pelleted by centrifugation at 4000 r.p.m. for 20 min at 4°C and resuspended in 30 ml BBS buffer (0.2 M boric acid, 0.16 M NaCl, pH 8.0) on ice. The cells were ruptured by passage through a French pressure cell three times and centrifuged at 20 000 r.p.m. for 15 min. The supernatant was then passed through a 0.22 µM filter and the filtrate was loaded onto a PC-Sepharose 4B column. The column was run in BBS buffer with a flow rate of 1 ml/min and elution was carried out with 10 ml BBS buffer containing 5 mM PC. Aliquots of all fractions were stored at 20°C for analysis by SDSPAGE and immunoblotting as described above.
Screening for antigen binding in solution
This method was modelled on that of Kazemier and co-workers (1996) and the affinity chromatography described above. Bacterial cultures were induced for protein production exactly as described above. Following pelleting of cells and resuspension in BBS buffer at a volume of 0.01xOD550 at the time of harvesting, the cells were subjected to head-over-head rotation for 1 h at 4°C. After centrifugation at 20 000 r.p.m. for 15 min and passage of the supernatant through a 0.22 µM filter, 0.4 ml of the cell preparation was added to 0.6 ml PC-Sepharose in BBS in a 2 ml Eppendorf tube. Incubation was at 4°C for 1 h with head-over-head rotation. The PC-Sepharose resin was then washed by brief centrifugation in a microfuge, removal of supernatant, and re-addition of 0.4 ml BBS buffer. After five such washes, 0.4 ml BBS buffer containing 12.5 mM PC was added and the resin was incubated at 4°C for 30 min with head-over-head rotation. To check the specificity of the binding, this procedure was carried out in duplicate, with one of the cell preparations incubated with 10 mM PC for 30 min prior to incubation with the PC-Sepharose resin. The supernatant fractions from the washing and elution steps were analysed by SDSPAGE and Coomassie blue staining or immunoblotting.
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Results |
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Sequence alignment of the VH genes of the two anti-PC antibodies reveals that the only differences between the McPC603 and T15 VH genes occur in the CDR2 and CDR3 regions (Figure 1). We therefore replaced VH CDR2 (according to the structural definition, see above and Figure 1
) or VH CDR3 from the T15 wild-type and framework-mutated antibodies with the corresponding CDR(s) from the antibody McPC603. Those residues differing from wild type in the grafted antibodies are highlighted in Figure 2
. These newly-mutated fragments were then analysed as before: to determine the physiology of the host bacterial cells producing them and their in vivo solubility, used as a measure of folding efficiency. The results of these experiments are represented in Figure 5
. It was found that the introduction of CDR-H3 from McPC603 into the wild-type Fv fragment had little effect on the host cells (Figures 5a and b
). Introduction of the same CDR into the H11 mutant version of the same fragment, however, led to a somewhat improved growth physiology compared to cells expressing the H11 fragments. This improvement upon introduction of McPC603 VH CDR3 was also seen in the M167 (H11) Fv fragment, at a much more pronounced level (not shown); no improvement was seen when the McPC603 VH CDR3 was introduced into the M167 wild-type fragment. Analysis of the folding of the improved fragments, carrying the CDR-H3 from McPC603, (T15 Fv fragments shown in Figure 4
) revealed that the proportion of soluble protein had increased significantly over that seen with the T15-H11 proteins. In contrast, the introduction of McPC603 VH CDR3 to the wild-type T15 Fv fragment resulted in soluble and insoluble protein levels the same as in the case of the wild-type fragment (not shown). It follows that the H11 mutations are required to see the beneficial effects of CDR-H3.
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Sequence alignment of the VL domains of McPC603 and T15 (Figure 1), carried out in a further search for determinants of poor folding in the T15 antibody fragments, led to 5 amino acid residues in the FW1 of T15 VL, which are different to the corresponding region in VL of McPC603 sequence (T9S, F10S, A12S, T14S and S16G; Figure 2
) being exchanged together. To examine the effect of this mutagenesis on functional binding, a miniaturized functionality assay was developed. Since the affinity is too weak for a monovalent fragment to survive the washing steps of an ELISA, PC-resin, as used for affinity chromatography, was incubated with the bacterial supernatant and then centrifuged and washed. In this resin, the ligand concentration is millimolar and thus, the monovalent fragment remains in the resin phase upon washing. To eliminate non-specific binding as a possible source of errors, controls were incubated in 10 mM PC before adding the PC-resin. The bound fragment was analysed by SDSPAGE.
The VL FRI-mutations were first introduced in a T15H11 VH background, resulting in the detection of this scFv by the PC-resin procedure outlined. The same protein was produced in a 2 l E.coli culture and purified by traditional affinity chromatography, the result of which is shown in Figure 6. This protein was quantified as approximately 200 µg. The mutant light chain was then cloned into vectors encoding the T15 wild-type and H11-McPC603 CDR3 heavy chain constructs. These proteins were expressed and assayed for PC binding as before. Both were found to be produced in functional form and each could be purified at 30 µg/2 l culture. None of the corresponding fragments with the original T15 VL could be shown to bind antigen or to be purifiable using either this procedure or traditional affinity chromatography. This shows that these VL mutations are a prerequisite to purify any functional T15 fragment, and to observe any other beneficial mutations in VH at the level of purifiable protein.
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Discussion |
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T15 antibody fragments, previously found in our laboratory to be produced in a non-functional form and to be extremely susceptible to protease-degradation in E.coli, were first mutagenized to introduce the `H11' triple mutation of the VH framework (Knappik and Plückthun, 1995). This mutation had been shown to improve the physiology of E.coli cells producing fragments of the related anti-PC antibody, McPC603, and the folding efficiency of the fragments themselves. This manipulation was found to significantly improve the folding of T15 Fv and scFv fragments, with a greater proportion of the mutated proteins being produced in soluble form than in the case of the wild-type proteins (Figure 4
). The apparent toxicity of the mutated fragments to E.coli was also reduced, as judged by the lower level of periplasmic leakiness and delayed lysis of the cells producing the fragments (Figure 3
); nevertheless, the levels of mutated McPC603 antibody fragments were not reached in either category.
Since the VL genes are quite dissimilar and are derived from different V genes (Perlmutter et al., 1984
; Malipiero et al., 1987
; Figure 1
), the VH gene of T15 was combined with the VL gene from each of the T15, M167, McPC603, and the extremely well-folding huMab4D5 antibody (Plückthun and Pfitzinger, 1991
; Carter et al., 1992
). As the toxicity of the fragments to the host cell was lowest when the T15 VH was expressed in combination with its original VL however (data not shown), it appeared that the other VL domains form only weak complexes with the T15 VH and do not rescue the VH into a soluble Fv fragment.
The subsequent CDR exchange experiments, in which we replaced VH CDR2 (according to the structural definition) or VH CDR3 in the T15 fragments with the corresponding CDR(s) from the better-folding McPC603 fragment, demonstrated that mutations in the T15 fragments do not simply have additive or synergistic effects, but rather, there is a hierarchy of their effects. Introduction of the McPC603 VH CDR3 into the H11 mutant of the T15 antibody led to a further improvement in the solubility of the antibody fragments (Figure 4) and, to a lesser extent, in the growth of the host E.coli cells (Figure 5
). However, this improved folding and solubility was seen in T15 fragments (and in M167 fragments) only upon prior introduction of the H11 framework mutations. In the absence of the framework mutations, therefore, the predominant pathway of periplasmic folding leads to aggregation and the composition of CDR-H3 only begins to have an effect when this diversion to aggregation has previously been overcome. This observed hierarchical effect of the manipulations also starts to explain the context dependence phenomenon of the effects of mutations in antibody fragments such as these.
Introduction of the McPC603 CDR-H2 into T15 can be seen to have no effect on host cell physiology in the H11 version and to have a negative effect in the wild-type fragment. This suggests that the wild-type fragment cannot tolerate additional problems associated with the imposition of the McPC603 CDR, whereas the H11 mutant, while not suffering any further disadvantage due to introduction of the new VH CDR2, gains no advantage from it. It is likely that the mutations A52G and D54K facilitate the aggregation involving positions 60 and 61 even further.
Finally, while the level of soluble protein being produced was greatly increased by this rational mutagenesis of T15 VH and the host bacterial cells showed a greatly stabilized physiology, none of the engineered fragments could be purified by affinity chromatography or using their peptide tag. This was thought to be due to their being produced in the bacteria in a soluble but non-functional form, the exact nature of which is unclear and is the subject of an ongoing study to characterize it precisely. Because the T15 VH domain has been converted entirely to VH of McPC603-H11 in this investigation, and because the Fv fragment McPC603-H11 (with its original VL domain) is easily purifiable by affinity chromatography, we chose to re-visit the VL domain in an attempt to restore the functionality of the T15 fragments.
The mutagenesis of the VL FW1 region was designed with a view to identifying key residue(s) in the T15 VL gene that were responsible for the lack of functionality of the Fv and scFv fragments, by exchanging them for the corresponding residues in the antibody McPC603. The T15 VH FW1 sequence TFLAVTAS (Figures 1, 2) was, therefore, mutated to SSLSVSAG. Affinity chromatographic screening of the H11 heavy chain mutant containing this altered light chain led to the purification of a protein band of the expected size. It is important to note that no improvement had been observed upon exchange of the whole VL domain of McPC603 (see above), since several VL residues need to contact the antigen and to make crucial interdomain hydrogen bonds (Satow et al., 1986
). Of the five residues changed in our analysis, modelling work indicated that the original Phe10 occurs in an exposed location at the bottom of the T15 VL domain (Figure 2
), where its replacement by a serine might be expected to disfavour aggregation. We propose that this residue in the T15 VL domain had previously been limiting the functionality of antibody fragments produced in E.coli and that it was only upon overcoming this problem that functional, affinity-purifiable fragments of the antibody could be produced for the first time. While the major effect of the mutation in this case was to restore functionality, the same mutation has also been observed by other workers to result in increased production in E.coli of an already functional Fab fragment (Forsberg et al., 1997
).
While the introduction of the FR1 mutations into VL by itself led to the production of a low level of functional protein, the H11 mutations in the VH, in the presence of the manipulated VL, then increased the level of affinity purifiable scFv produced by a factor of 7. In the case of the H11-McPC603 CDR3 scFv, the reduced level of purifiable protein is probably due to a perturbation in the binding pocket upon grafting of the McPC603 VH CDR3 to T15, resulting in a reduction in the affinity of the fragment.
We conclude that this work demonstrates that there is a hierarchy of factors influencing the folding of recombinant antibody fragments produced in E.coli. The effectiveness of the structured approach we have employed is such that even previously non-functional antibodies can be engineered into well folding molecules. Furthermore, this analysis of the hierarchy of events should be informative in delineating the molecular mechanisms of aggregation.
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Acknowledgments |
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Notes |
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References |
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Received July 23, 1998; revised January 25, 1999; accepted March 22, 1999.