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Parvalbumins in 21 common finfish species : presence and the effect of processing on immunoreactivity /Gazzaz, Sahl Sadagah. January 1992 (has links)
Thesis (Ph. D.)--University of Washington, 1992. / Vita. Includes bibliographical references (leaves [264]-282).
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Identification and characterisation of specific allergens of Abalone (haliotis midae; mollusca) and other seafood speciesLopata, Andreas L January 1999 (has links)
Shellfish and fish are sources of potent allergens in sensitised individuals. In view of the limited information available from published studies, especially on mollusc allergens, more detailed characterisation of the major allergens from different shellfish and fish is necessary to accurately predict cross-allergenicity. The need for a detailed characterisation of the immune response and the allergens in an indigenous mollusc species, followed a recent increase in patients presenting in the Cape Town area, with TY.pe I allergic reactions after ingestion of abalone (Haliotis midae). The first objective of this study was to determine the frequency and spectrum of reported hypersensitivity to abalone and other related seafood species in the Western Cape of South Africa. 105 volunteer subjects with suspected seafood allergy were recruited by means of a detailed seafood allergy questionnaire, advertised in the local press. The analysis of the questionnaire demonstrated clearly the importance of abalone, which was the third most frequently reported species (35%), after rock lobster and shrimp, of the 26 seafood species implicated in allergic reactions. Allergy to seafood was confirmed by the presence of specific IgE using in-house and commercial radioimmunoassays (RASTs). A novel Abalone-RAST identified specific IgE to abalone in 17/38 subjects who reported adverse reaction following the ingestion of abalone. The novel Abalone-RAST correlated positively not only with the phylogenetic closely related Snail-RAST (p<0.01) but also with squid and several indigenous crustacean species. Among subjects with multiple seafood allergies, the immune responses to molluscs species were found to be diverse. The presence of species specific allergens in the mollusc group was supported by the very low frequency of concurrent sensitivity to all mollusc species (13%) compared to concurrent sensitivity between mollusc and among the crustacea and fish group (42% and 56% respectively). The persistence of specific IgE, following a period of more than three years of seafood avoidance, was demonstrated in the mollusc species studied. The second objective was to investigate the specific immune responses to local seafood in more detail using RAST-inhibition experiments, skin prick tests (SPTs) and Western blots to demonstrate the presence of species-specific allergens. Sensitivity for the detection of abalone allergy was improved using an additional in-house SPT in six RAST negative subjects (23/38, 61 %). RAST-inhibition experiments with abalone extract demonstrated the highest degree of cross-reactivity with the Snail-RAST. In addition, a strong inhibition was achieved using commercial crustacean RASTs, confirming the presence of cross-reacting allergens in species of the same and other seafood groups. However, the low inhibitions achieved with the indigenous black mussel and squid extracts indicated that their allergen compositions differ from the species utilised in the commercial RASTs. Unique species-specific protein bands could be detected by SDS-gel electrophoresis, which clearly distinguished related mollusc species. These have not been demonstrated previously. Western blot analysis of different mollusc species identified several prominent allergens. An unexpected finding was the appearance of novel specific IgE binding reactivity after cooking the abalone. Several IgE binding proteins with similar molecular weights could be detected in immuno blots of indigenous crustacean and fish species. The next objective was to characterise the hypersensitive reactions to the local abalone species (H midae) in detail and identify the allergens found in this mollusc species. The questionnaire on abalone sensitive subjects revealed that asthma-like symptoms and the delayed onset of symptoms were frequent in sensitised individuals (42% and 34% respectively). This has previously only been reported for snail and in one case report on abalone. Surprisingly, the five abalone sensitive subjects who were studied in more detail had concurrent sensitivity to HDM and, analysed by RAST-inhibition, demonstrated two distinct types of responses. One set of subjects demonstrated a strong inhibition by HDM, indicating clearly for the first time that cross-reacting allergens or epitopes must exist between the food allergens from abalone and the air borne allergens found in HDM. SDS-gel electrophoresis demonstrated common but in addition species-specific protein bands even between very closely related abalone species from South Africa, Australia and Japan. Western blot analysis revealed two major allergens with molecular weights of about 38 and 45 kDa. Their remarkable thermal stability was demonstrated by various in-vitro and in-vivo assays. These two allergens were also present in extracts of other indigenous mollusc species, and surprisingly in some local crustacean and fish species. The individual immune responses to mollusc species were very heterogeneous for each analysed individual. The 38 kDa allergen is believed to belong to the protein family of tropomyosins, as was supported by specific IgE binding to recombinant tropomyosin of shrimp. This novel 45 kDa allergen of the South African abalone (H midae), was registered with the WHO International Union of Immunological Societies (IUIS) as Hal m 1. It is only the second allergen recognised for a mollusc species after Tod p 1 from squid. A further aim of these studies was to generate monoclonal antibodies (MoAbs) to the mollusc allergens using the hybridoma technology. The MoAbs were used, due to their consistent specific binding, to identify cross-reacting allergens among species of different seafood groups. In addition, I attempted to develop an immunologic test to distinguish between abalone species from different parts of the world. This test is of importance for the South African police to identify for forensic purposes unequivocally, fresh or processed abalone tissue exported illegally from South Africa to the Far East. Three ELISA- and Western blot assay positive clones were analysed. They demonstrated highly individual binding profiles when binding to fresh and cooked mollusc species was analysed. MoAb clones 2.11 and 2.12 (generated to the same protein of abalone) lacked complete binding to four and two of the ten abalone species respectively, allowing for very distinct species identification. Furthermore, antibody binding to cross-reacting proteins in crustacea and fish was also detected. Western blot results demonstrated clearly that these two antibodies bind to different epitopes on the same protein, making them very useful as tool for allergen and species identification. Finally, an amino acid analysis of the 3 purified antibody binding fractions of abalone was conducted. These proteins were rich in glutamine and asparagine, like tropomyosin, but differed significantly from tropomyosin with respect to serine content. The immunological findings using different patient specific sera and the monoclonal antibodies generated, provide important new information and insights into the concordant and multiple positive sensitivity to molluscs, crustacea and fish, and new information about the complexity and stability of immune responses to seafood and mollusc allergens observed in allergic subjects.
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Characterisation of allergens in pilchard, responsible for the development of occupational allergy in the seafood processing industry in the Western CapeHikuam, Christopher Willem January 2006 (has links)
Thesis (MTech (Tourism and Hospitality Management))--Cape Peninsula University of Technology, 2006. / The increase in popularity of fish, coupled with technological advances in the
fishing industry and changes in the control and management of fishing resources,
has led to a significant increase of fish processing workers from 13 million in
1970 to 38 million in 2002. Whereas allergic reactions to fish proteins were
previously only documented in consumers, increasing reports of occupational fish
allergies of fish processing workers has become evident. In South Africa, the
reported prevalence of occupational asthma associated with fish processing
workers is 2 - 8%, and the prevalence of occupational protein contact dermatitis
3 - 11%. Pilchard is one of the most consumed fish species in South Africa and
the immunological analysis of this species will therefore contribute to the
provision of occupational health services in the pilchard processing industry.
Proteins extracted from fresh, frozen and canned pilchard (Sardinops sagax), as
well as fresh samples of six other processed and consumed South African fish
were characterised by denaturing protein electrophoresis and immunoblotted with
different monoclonal and polyclonal antibodies. Sera from sensitised workers
were subsequently used to characterise the membrane-bound pilchard proteins
and analysed for human Immunoglobulin G (lgG) and Immunoglobulin E (IgE)
antibodies to determine antigen recognition.
A protein of 12 kDa molecular weight was found to be present in all fish protein
extracts, however, at various concentrations. With the aid of the monoclonal and polyclonal antibodies, the 12 kDa protein was postulated to be parvalbumin, a
known allergen in some fish species. Immunoblotting experiments for the
identification of workers' IgG- and IgE-reactivities to fresh, frozen and canned
pilchard showed a 12 kDa protein as an immunolgically reactive fish protein.
This protein was also found to occur in dimeric, trimeric and tetrameric forms,
which may have significant implications in the diagnosis and management of
occupational sensitisation to pilchard.
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Immunological techniques for the serum determination of specific-IgE levels among workers exposed to seafood allergensElliott, Alicia Rochelle January 2003 (has links)
Thesis (MTech (Biomedical Technology))--Cape Technikon, 2003 / Allergic conditions among workers processing seafood are most often related to inhalation of
the seafood antigens or via direct unprotected handling of the seafood and its products. This
can cause sensitised individuals to suffer from asthma, rhino-conjunctivitis, urticaria and
protein contact dermatitis, which are IgE mediated. Food intolerance may also occur which is
a non-IgE mediated reaction, however the exact mechanism is yet to be determined. There is
therefore a need to develop reliable tests to identify sensitised workers processing seafood.
The objective of this study was to prepare specific seafood extracts from raw and cooked
lobster; raw and cooked saltwater bony fish species (mackerel, red eye, maasbanker, pilchard
and anchovy) and fishmeal dust obtained from a fish-processing factory. These extracts were
tested by SDS-Polyacrylamide Gel Electrophoresis to characterise the seafood proteins, and
the allergenicity was confirmed by the Western blot technique. Polyclonal IgG antibodies
were also successfully generated in rabbits, using the specific seafood extracts isolated from
the various species.
The second objective was to optimise and standardize an Enzyme Allergosorbent Test
(EAST) method to quantify specific IgE antibodies in the sera of factory workers. This EAST
was optimised and validated to detect allergen-specific IgE to each of the different fish
species and also one crustacean species (rock lobster). Sera from a group of workers were
selected and analysed for specific IgE antibodies by the optimised EAST (S) (South African
laboratory), and commercial RAST techniques. Analysis was performed for the three most
important extracts, pilchard (canned), anchovy, and lobster. The same samples were analysed
by EAST (R) in the reference laboratory (Dr Gerald Reese; Paul-Ehrlich-Institute, Germany).
The different techniques, and the EAST (R) and the EAST (S) results were compared by
using a statistical software package.
An EAST method was successfully developed, however, compared to the results obtained by
the reference laboratory the sensitivity and specificity was below 80%. The main reason for
the low agreement between the two laboratories was the fact that the South African laboratory
used a modified EAST method, and different data calculation methods, for categorising
positive results. The South African laboratory did not use a kit-based assay and a serum
dilution of 1:4 and not 1:2 were used when compared to the reference laboratory. When the
EAST results were compared to the RAST results, poor agreement was found due to the fact
that canned pilchard was used in the EAST while raw pilchard in the commercial RAST
assay. For pilchard, anchovy and lobster EAST, different species were utilized compared to
the RAST, and this can also explain the poor level of agreement.
Future directions would be to further standardise the EAST method and to introduce reference
sera and a standard curve to determine positive results, thereby ensuring more reproducible
results between laboratories.
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