Many studies noted that LAB were on

Many studies noted that LAB were one of the main constituents
of the normal indigenous flora of human, which contributed several
health benefits including improvement of intestinal tract health,
enhancing the immune system, reducing risk of certain cancers,
lowering serum cholesterol concentrations, reducing blood pressure
Chen-Kai Chang et al./Asian Pac J Trop Biomed 2015; 5(4): 281-286 285
in hypertensives, reducing dental caries, and improving female
urogenital infections and Helicobacter pylori infections[1,2,15].
Evidence from clinical and animal studies has supported that some
LAB can modify immune response of the host[16,17]. In order to
evaluate whether selected strains are able to induce the production
of inflammatory responses, we examined the ability of the selected
strains to induce cytokines secretion by macrophages. Macrophages,
taking part in both innate and adaptive immune responses, are
derived from monocytes[18]. Once macrophages are activated, they
can phagocytose microorganism, secrete proinflammatory cytokines,
and present antigens to helper T cells. Many of these activities are
medicated through the release of different cytokines[18,19]. For
instance, macrophages in the presence of pathogen can produce
NO to kill the antigen, and secrete cytokines such as IL-6 and
TNF-α that activate specific immune[20]. In the present work, strains
B0040, B0110 and B0145 induced significant NO production of
macrophages. These findings suggested that the possible way of
NO production of macrophages treated with strains B0040, B0110
and B0145 may be through the L-arginine pathway[21]. The role
of NO in intestinal inflammation is controversial. In physiological
amount, it plays a crucial and protective role in human defense
systems, whereas overexpression of NO during inflammation may
lead to cytotoxity[21]. The result shows that the NO production of
macrophages induced by the selected strains B0040, B0110, and
B0145 is less than that of LPS treatment and higher than L. casei.
Clearly, the NO production of macrophages induced by the selected
strains appears to induce positive immune response. In addition,
small amounts of NO may stimulate mitochondrial biogenesis and
boost the supply amount of oxygen and respiratory substrates to
mitochondria. Thus, the use of the selected strains that are able to
produce appropriate levels of NO may potentially enhance immune
response. Production of TNF-α in macrophage cells that were
stimulated with the selected strains was induced in amounts even
greater than those treated with LPS, indicating that strains B0040
and B0145 were capable of inducing RAW 264.7 cells to secrete
higher levels of TNF-α production. As for IL-6, it is critical to
mucosal immunity based on its effects on the differentiation of IgAcommitted
B cells and its production in the gut by macrophage, T
cells and other cells[10,22]. In this work, we demonstrated the ability
of the selected strains to induce the production of IL-6 in RAW 264.7
cells, in modulation of the immune response of the host. Moreover,
IL-6 production in the cells stimulated with the selected strains gave
rise to much higher levels than L. casei. These observations suggest
that IgA in the cells induced by the selected strains may increase,
thereby facilitating the modulation of the immune response of the
host.
Among the strains tested, viable cells were better inducers than
heat-inactivated strains or LAB-SCS in production of NO and
TNF-α. Similarly, the heat-inactivated bacteria and LAB-SCS could
induce NO and cytokines production, such as IL-6 and TNF-α, in
macrophage cell line RAW 264.7, indicating that viable, nonviable
(heat-inactivated) or LAB-SCS can induce the immunopotentiating
activities. Cell-free cultures of LAB with probiotic potentials
demonstrated to exert antimicrobial and immunomodulatory
activities, suggesting the use of probiotic in nonviable forms[23].
Increasing evidence showed that cell wall fragments of bacteria,
their metabolites and dead bacteria could elicit immune responses.
Chiang et al. have reported immunomodulation effects of dead
lactobacilli, whole cells and gastrointestinal enzymatic hydrolysates
of supernatants and precipitates from Lactobacillus paracasei subsp.
paracasei NTU 101, on RAW 264.7 macrophages and splenocytes[24].
We suggested that the induction of heat-inactivated cells or LABSCS
on macrophages may result from the intact bacterial cells
components or metabolites in LAB such as peptidoglycan, teichoic
acid and exopolysaccharide[25,26]. However, further in vivo
verification is needed.
In conclusion, the present study indicated that strains B0040,
B0110 and B0145 did activate macrophage RAW 264.7 to stimulate
NO and pro-inflammatory cytokines production. We suggest that
strains B0040 and B0110, identified as Lactobacillus plantarum,
and B0145, as Weissella cibaria, may be potential candidates for
supplement to induce immunopotentiating activities. However,
further in vivo verification is necessary