Histocompatibility testing refers t

Histocompatibility testing refers to the determination of tissue antigens
and their immunologic reactions. Testing includes isolation of cells such
as lymphocytes, platelets, granulocytes and other tissue cells, HLA typing
for A, B, C, DR and DQ locus antigens, antibody detection, crossmatching
and mixed lymphocyte culture.
Terminology of HLA antigens should conform to the nomenclature
adopted by the World Health Organisation.
REAGENTS
HLA typing reagents
Well characterised HLA typing antisera of confirmed specificity procured
from commercial firms and reference laboratories should be used for
HLA typing.
HLA typing reagents should be stored at -300C or below either in bulk or
loaded in typing trays.
Control sera
Each typing or crossmatching should be carried out with appropriate
controls which include complement dependent positive controls and
negative controls(neutral AB serum).
Cell viability in negative control well at the end of incubation should
permit accurate interpretation of results. The positive and negative
control should give cytotoxicity results of 80% and less than 15%
respectively.
Complement should be stored in small aliquotes either in lyophilised
state or in liquid form at below -300C.
Each new batch of complement should be tested for its potency to
induce cytotoxicity in the presence of specific antibody, but is not cytotoxic
to the test cells in the absence of specific antibody.
HLA TYPING
Typing for each of the antigens for HLA - A, B, C and DR & DQ loci should
be defined by atleast two antisera, one of which is monospecific.
HLA typing should be performed by complement dependent micro
lymphocytotoxicity method or by other equally sensitive tests.