During the past two decades, there have been numerous attempts at using animals
in order to produce recombinant human proteins and monoclonal antibodies.
However, it is only recently that the first two therapeutic agents isolated
from the milk of transgenic animals, C1 inhibitor (Ruconest) and antithrombin
(ATryn), appeared on the market. This inspires hope that a considerable number
of new recombinant proteins created using such technology could become
available for practical use in the near future. In this review, the methods
applied to produce transgenic animals are described and the advantages and
drawbacks related to their use for producing recombinant human proteins and
monoclonal antibodies are discussed.
In this study, we investigated the possibility of phototoxic flavoprotein
miniSOG (photosensitizer) excitation in cancer cells by bioluminescence
occurring when luciferase NanoLuc oxidizes its substrate, furimazine. We have
shown that the phototoxic flavoprotein miniSOG expressed in eukaryotic cells in
fusion with NanoLuc luciferase is activated in the presence of its substrate,
furimazine. Upon such condition, miniSOG possesses photoinduced cytotoxicity
and causes a 48% cell death level in a stably transfected cell line.
Tissue renewal is a well-known phenomenon by which old and dying-off cells of various tissues of the body are replaced by progeny of local or circulating stem cells (SCs). An interesting question is whether donor SCs are capable to prolong the lifespan of an aging organism by tissue renewal. In this work, we investigated the possible use of bone marrow (BM) SC for lifespan extension. To this purpose, chimeric C57BL/6 mice were created by transplanting BM from young 1.5-month-old donors to 21.5-month-old recipients. Transplantation was carried out by means of a recently developed method which allowed to transplant without myeloablation up to 1.5 × 108 cells, that is, about 25% of the total BM cells of the mouse. As a result, the mean survival time, counting from the age of 21.5 months, the start of the experiment, was +3.6 and +5.0 (±0.1) months for the control and experimental groups, respectively, corresponding to a 39 ± 4% increase in the experimental group over the control. In earlier studies on BM transplantation, a considerably smaller quantity of donor cells (5 × 106) was used, about 1% of the total own BM cells. The recipients before transplantation were exposed to a lethal (for control animals) X-ray dose which eliminated the possibility of studying the lifespan extension by this method.
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