2015
DOI: 10.1007/s00216-015-8889-6
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Heavy chain single-domain antibodies to detect native human soluble epoxide hydrolase

Abstract: The soluble epoxide hydrolase (sEH) is a potential pharmacological target for treating hypertension, vascular inflammation, pain, cancer and other diseases. However, there is not a simple, inexpensive and reliable method to estimate levels of active sEH in tissues. Toward developing such an assay, a polyclonal-variable domain of heavy chain antibody (VHH) sandwich immunoassay was developed. Ten VHHs, which are highly selective for native human sEH, were isolated from a phage displayed library. The ten VHHs hav… Show more

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Cited by 14 publications
(25 citation statements)
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“…The VHH phage display library was built as previously described 4,25 . A three-year-old llama ( Lama glama ) from the Montevideo municipal zoo was immunized every two weeks with 6 doses of 500 µg of recombinant, affinity purified human sEH in incomplete Freund adjuvant by sub-cutaneous injection.…”
Section: Methodsmentioning
confidence: 99%
“…The VHH phage display library was built as previously described 4,25 . A three-year-old llama ( Lama glama ) from the Montevideo municipal zoo was immunized every two weeks with 6 doses of 500 µg of recombinant, affinity purified human sEH in incomplete Freund adjuvant by sub-cutaneous injection.…”
Section: Methodsmentioning
confidence: 99%
“…Furthermore, because VHH has only one variable region, specific antibodies can be screened at 1x10 6 . However, in ordinary antibody Fab or ScFv libraries, the library needs to be large enough to more easily screen for antibodies (93,96,97,102,103).…”
Section: Construction Of Library and Panning Of Nanobodiesmentioning
confidence: 99%
“…The phage display technology is used to screen binders for various targets from diverse and large libraries and is widely employed by various research teams. Since the difference between VHH and VH is mainly due to the absence of the CH1 region, the work of building an immune and natural library focuses on isolating antibodies lacking CH1 from IgG, which can be achieved by one-step ( 96 ) or two-step nested PCR amplification ( 97 ). The key of PCR is to design PCR primers using the conserved nucleotide sequence of the antibody back-bone region.…”
Section: Construction Of Library and Panning Of Nanobodiesmentioning
confidence: 99%
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