Transposon Mutagenesis of Probiotic Lactobacillus casei Identifies asnH, an Asparagine Synthetase Gene Involved in Its Immune-Activating Capacity

Lactobacillus casei ATCC 27139 enhances host innate immunity, and the J1 phage-resistant mutants of this strain lose the activity. A transposon insertion mutant library of L. casei ATCC 27139 was constructed, and nine J1 phage-resistant mutants out of them were obtained. Cloning and sequencing analyses identified three independent genes that were disrupted by insertion of the transposon element: asnH, encoding asparagine synthetase, and dnaJ and dnaK, encoding the molecular chaperones DnaJ and DnaK, respectively. Using an in vivo mouse model of Listeria infection, only asnH mutant showed deficiency in their ability to enhance host innate immunity, and complementation of the mutation by introduction of the wild-type asnH in the mutant strain recovered the immuno-augmenting activity. AsnH protein exhibited asparagine synthetase activity when the lysozyme-treated cell wall extracts of L. casei ATCC 27139 was added as substrate. The asnH mutants lost the thick and rigid peptidoglycan features that are characteristic to the wild-type cells, indicating that AsnH of L. casei is involved in peptidoglycan biosynthesis. These results indicate that asnH is required for the construction of the peptidoglycan composition involved in the immune-activating capacity of L. casei ATCC 27139.


Introduction
Probiotics are defined as live microorganisms which, when administered in sufficient amounts, confer health benefits in the host in addition to their nutritional effects [1]. Among the various health-promoting functions of the probiotics, much attention has been paid to their immune regulatory activity, since they are often used both in clinical applications and as foods that function to maintain the immunologic homeostasis of the host [1,2].
Lactobacilli are the normal commensals in the human intestines, and certain Lactobacillus strains are regarded as probiotic bacteria. L. casei strain Shirota has been widely studied for its probiotic effects including immunomodulating activity. It enhances NK cell activity by dairy intake [3,4] and prevents and reduces the risk of recurrence of bladder cancer by oral administration in human [5,6]. In addition, this strain also enhances anti-infectious activity against Listeria monocytogenes [7,8] and Pseudomonas aeruginosa [9] and inhibits the growth of transplantable allogeneic and syngeneic mouse tumors in several experimental animal models [10][11][12][13][14]. However, the detailed molecular mechanisms involved in these processes have not been understood.
L. casei ATCC 27139, the parental strain of Shirota [15], has been consistently shown to exhibit anti-infectious activity against L. monocytogenes and anti-tumor activity against MethA fibrosarcoma in mice associated with the marked increases in the cytokine levels such as TNF-a, IL-12, IL-18, and IFN-c [16]. Although L. casei ATCC 27139 is susceptible to J1 phage, which shows a remarkably high specificity to certain strains of L. casei/L. paracasei [17], J1 phage-resistant mutants of this strain have been reported to be deficient in the immune-activating capacity [16], suggesting that the bacterial components associated with J1 phage sensitivity may be related to the activity. Despite the probable relationship between the J1 phage sensitivity and the immune-activating capacity of this strain, the genetic determinants responsible for J1 phage resistance have not been identified because of the technical limitation of the introduction of mutagenesis using chemical mutagen.
Recently, we developed a random mutagenesis system using a Tn5-based EZ::TN transposome for the probiotic L. casei ATCC 27139 [18]. Using this system, we constructed a Tn5 insertion library of nearly 10,000 transposon insertion mutants of L. casei ATCC 27139 that represents the first genome-wide random mutagenesis approach for lactobacilli [18]. Analysis of the transposon insertion mutants by Southern hybridization and sequencing of transposon insertion sites confirmed non-biased transposon insertion events [18]. Using a part of the Tn5 insertion library, we have identified the genes responsible for amino acid auxotrophy, glycine or alanine biosynthesis, respectively, which further allowed the validation of the usefulness of this library [18].
In this study, we describe the identification of the gene required both for the J1 phage sensitivity and the immune-activating capacity of L. casei ATCC 27139 using a Tn5 insertion library. In addition, correlation between probiotic function of L. casei ATCC 27139 and cell wall structure was studied.

Materials and Methods
Bacterial strains, phage, and growth conditions L. casei ATCC 27139 was used as the wild-type strain. Lactobacilli were cultured in ILS medium [18]. The virulent L. monocytogenes strain EGD, was grown in brain heart infusion medium (Becton Dickinson and Co., Franklin Lakes, NJ) prior to infecting the mice. Escherichia coli JM109 was used as the host organism for molecular cloning and expression of recombinant proteins. E. coli strains were cultured in Luria-Bertani (LB) medium.
A random transposon mutant library was generated using an Tn5 transposon insertion as described previously [18]. A total of nearly 10,000 mutants were arrayed in a 96-well plate and stored at 280uC in 40% glycerol.
J1 phage was obtained from the American Type Culture Collection (ATCC 27139-B1). After many rounds of phage multiplication in L. casei ATCC 27139, a J1 phage lysate was prepared and used for infection as described previously [16,18]. If required, the following antibiotic concentrations were used: 25 mg/ml of erythromycin for lactobacilli, 500 mg/ml of erythromycin for E. coli, 10 mg/ml of chloramphenicol for lactobacilli and E. coli, and 100 mg/ml of ampicillin for E. coli.
Screening of Tn5 insertion mutants for the J1 phage-resistant phenotype Tn5 insertion mutants were screened for their level of J1 phage resistance compared with the wild-type strain as the parental control. Mutants were inoculated into ILS broth containing J1 phage lysate at a multiplicity of infection (moi) of 10 using a 96well plate. After incubation at 37uC for 48 h, the mutants grown in ILS broth containing J1 phage were regarded as resistant to J1 phage. To ascertain the resistance levels of the mutants to J1 phage infection, the cells of the wild-type strain and the mutants were mixed with J1 phage in ILS broth at an moi of 0.5, and the number of PFU was counted after incubation at 37uC for 24 h. Relative J1 phage sensitivity was calculated as the ratio of PFU for transposon insertion mutants to that of the wild-type strain.

Analysis of DNA sequence and identification of the transposon insertion site
Self-ligation-mediated inverse PCR was used to characterize the Tn5 insertion site, as described previously [18]. In brief, NcoI-, BanII-, or KpnI-digested chromosomal DNA from the strain carrying the Tn5 insertion was self-ligated, and inverse PCRs were performed on ligated templates using a primer set of SqFP (59-GCCAACGACTACGCACTAGCCAAC-39) and SqRP (59-GAGCCAATATGCGAGAACACCCGAGAA-39). PCR products were sequenced, and the sequences were identified using the BLAST program (http://blast.ncbi.nlm.nih.gov/BLAST.cgi; NCBI, Bethesda, MD).

Experimental infection
Animal experiments were approved by the Kitasato University Institutional Animal Care and Use Committee (Permit Number: J10-1) and were performed in accordance with the Regulations for the Care and Use of Laboratory Animals in Kitasato University and with the National Research Council Guide for the Care and Use of Laboratory Animals in Japan. Specific pathogen-free male BALB/c mice (Charles River Japan, Kanagawa, Japan) were used for the mouse infection model as described previously [16]. Briefly, the mice were injected intravenously (i.v.) with a heat-killed preparation of lactobacilli (800 mg/mouse) 6 days before Listeria infection. The L. monocytogenes strain EGD (2.0610 6 CFU) was injected i.v. 6 days after lactobacilli inoculation. The number of viable Listeria in spleen homogenates 24 h after the challenge was counted; the plates containing the appropriate diluents of the homogenates were maintained at 37uC.

Cytokine detection by enzyme-linked immunosorbent assay (ELISA)
Heat-killed lactobacilli preparations (800 mg) were injected i.v. into mice. IL-12, TNF-a, and IFN-c were measured from spleen homogenates 8 h after the challenge using OptEIA TM ELISA kits (BD Biosciences Pharmingen, San Diego, CA) as described by the manufacturer. Absorbances were measured using a model 3550 microplate reader (Bio-Rad Laboratories, Hercules, CA). Sample data were extrapolated from standard curves using Microplate ManagerH 6 software (Bio-Rad Laboratories).
Expression and purification of recombinant proteins E. coli BL21 (TaKaRa Bio, Shiga, Japan) strains containing plasmids encoding FLAG fusion proteins were grown at 37uC in LB broth overnight. The cultures were diluted 1:100 into fresh LB broth supplemented with 0.4% (w/v) glucose and incubated at 25uC for 3 h. Isopropyl-b-D-thiogalactopyranoside was added to a final concentration of 1 mM, and the cultures were further incubated at 25uC for 5 h. To purify FLAG fusion proteins, bacteria were centrifuged at 70006g for 10 min at 4uC and resuspended in 10 ml of CelLytic B TM reagent (Sigma-Aldrich Co.) with cOmplete, Mini protease inhibitor cocktail tablets (Roche Diagnostics Co., Basel, Switzerland). After a 15 min incubation at room temperature, samples were centrifuged at 15,0006g for 20 min at 4uC to pellet cellular debris. FLAG fusion proteins were purified using an anti-FLAG M2 affinity gel according to manufacturer's instructions (Sigma-Aldrich Co.). Protein concentrations were quantified according to the Bradford method using the protein assay dye reagent concentrate (Bio-Rad Laboratories).

Enzymatic activity of AsnH
The enzymatic activity of AsnH was measured using an AmplexH Red Glutamic Acid/Glutamate Oxidase Assay Kit (Molecular Probes, Eugene, OR) according to the methods described previously [20]. Briefly, aspartic acid or cell wall extracts of L. casei ATCC 27139, used as the substrates, were diluted with a reaction mixture containing 50 mM Tris-HCl (pH 7.5), 15 mM MgCl 2 , 25 mM KCl, 1 mM glutamine, 0.2 mM dithiothreitol, and 2 mM ATP. Several concentrations of glutamic acid (0-20 mM) were used as the standard. Fifty microliters of the substrate solution were added to 50 ml of the AmplexH Red reagent/horse radish peroxidase/glutamate oxidase/glutamatepyruvate transaminase/alanine working solution. After incubation at 30uC for 30 min, luminescence was detected using a SpectraMax5 microplate reader (Molecular Devices Co., Sunnyvale, CA) with excitation at 544 nm and emission at 595 nm. Sample data were extrapolated from standard curves using Microplate ManagerH 6 software (Bio-Rad Laboratories).

Gram staining and transmission electron microscopy
Gram staining of L. casei cells grown to the early stationary phase in ILS broth was performed using Fiber G (Nissui Pharmaceutical Co.), in accordance with the manufacturer's recommendations, and the cells were observed using OLYMPUS BX50 light microscope (OLYMPUS Co., Tokyo, Japan). For transmission electron microscopy (TEM) analyses, L. casei cells were fixed with 2% glutaraldehyde in 100 mM phosphate buffer (pH 7.4), postfixed in osmium tetroxide at 4uC, dehydrated, and embedded in Epon 812 resin. Ultrathin sections were analyzed using JEM-1200EX TEM (JEOL, Tokyo, Japan) at 80 kV.

Preparation of cell wall extracts
Two-hundred-milliliter cultures of L. casei grown to the early stationary phase in ILS broth were centrifuged at 80006g at 4uC for 10 min. The cells were washed 3 times with distilled water and resuspended in 20 ml of acetone. Suspensions were centrifuged at 30006g at 4uC for 10 min, and precipitates were washed again with acetone and suspended in 10 ml of chloroform/methanol (2:1). Suspensions were incubated at 60uC for 30 min and centrifuged at 30006g at 4uC for 10 min. Precipitates were resuspended in 50 mM Tris-HCl (pH 7.0) with DNaseI and RNaseA at final concentrations of 1000 U and 50 ng/ml, respectively, and incubated at 37uC for 1 h. Proteinase K was added to the lysates to a final concentration of 1 mg/ml, and suspensions were heated at 37uC for 16 h. After centrifugation at 20,0006g at 4uC for 40 min, precipitates were washed with 50 mM Tris-HCl (pH 7.0) and treated with 0.1% (w/v) sodium dodecyl sulfate in distilled water at 100uC for 10 min. Suspensions were then centrifuged at 20,0006g at 4uC for 40 min, and precipitates were washed with distilled water 6 times. Precipitates were then washed with 20% (v/v) ethanol and 5% (w/v) NaCl 3 times and again with distilled water 3 times. After centrifugation at 20,0006g at 4uC for 40 min, precipitates were lyophilized and used as cell wall extracts.

Amino acid composition of the peptidoglycans
Cell wall extracts prepared as described above were suspended in 5 ml of 10% (v/v) trichloroacetic acid and heated at 100uC for 20 min. After centrifugation at 12,0006g at 4uC for 30 min, precipitates were washed 3 times with 50 mM phosphate buffer (pH 7.2) and then with 100% (v/v) ethanol. The resultant residues were suspended with diethyl ether and centrifuged at 15,0006g at 4uC for 10 min. Precipitates were lyophilized and used as the peptidoglycan fraction. The purified peptidoglycans (1 mg) were hydrolyzed in 6 N HCl at 100uC for 16 h, and the amino acid composition was analyzed by high-performance liquid chromatography using a Waters 2695 Separations Module (Waters co.,

Sensitivity to lysozyme
To ascertain the sensitivity of L. casei strains to lysozyme, L. casei ATCC 27139 and its mutants that had been pre-incubated in ILS broth at 37uC for 48 h were inoculated at 1.0610 7 CFU/ml into fresh ILS broth containing various lysozyme concentrations (0-10,000 mg/ml). Following incubation at 37uC for 48 h, the minimal inhibitory concentration of lysozyme at which L. casei strains failed to grow was regarded as its MIC.

Statistical analysis
The results of peptidoglycan thickness are presented as the means 6 standard error of the mean (SEM) and the others are presented as the means 6 standard deviations (SD) of triplicate experiments. Statistical analyses were performed using Student's t-test. Differences were considered significant at p,0.05.

Nucleotide sequence accession number
The sequence orthologs of the asnH gene were obtained from the DDBJ/EMBL/GenBank database. The accession numbers for the Rhodococcus erythropolis, Corynebacterium glutamicum, Mycobacterium smegmatis, and Escherichia coli sequences were AB183824, BX842579, AB183824, J05554, respectively, and GeneID of the  Lactococcus lactis was 4797108. The alignment was constructed using the GENETYX program (Genetyx Co., Tokyo, Japan).

Isolation of J1 phage-resistant mutants of L. casei ATCC 27139 from a random Tn5 insertion library
To identify genes involved in the augmentation of host innate immunity by L. casei, a total number of 9408 Tn5 insertion mutants from the mutant library were screened for their J1 phage sensitivity using a 96-well plate assay. Nine mutants (MT77, MT2890, MT3332, MT4156, MT5740, MT6674, MT7279, MT7398, and MT8105) displayed significantly higher resistance to J1 phage compared with the wild-type parental strain. Sensitivities to J1 phage infection of these mutants were 10 4 -fold lower than that of the wild-type strain (Table 1). Southern hybridization analyses confirmed that all these mutants carried a single independent Tn5 transposon insertion (data not shown).
The asnH mutant of L. casei ATCC 27139, but not the dnaJ or dnak mutants, is deficient in the immune-augmenting activity Since previous studies have demonstrated that the heat-killed preparation of J1 phage-resistant mutants of L. casei ATCC 27139 are deficient in the immune-augmenting activity, we assessed this activity in the J1 phage-resistant Tn5 mutants obtained in this study using a mouse model of Listeria infection. Whereas mice pretreated with L. casei dnaJ (MT3332) and dnak (MT7279) mutant strains exhibited anti-listerial activity comparable to that of the wild-type strain, the asnH mutant (MT77) showed no significant activity (Fig. 1A). The defect in anti-listerial activity in the asnH mutant resulted solely from the absence of asnH because significant protection against Listeria infection in mice could be restored to wild-type levels by introducing a plasmid harboring asnH into the mutant (Fig. 1B). As for the induction of innate cytokines such as IL-12, TNF-a, and IFN-c in the host, the asnH mutant did not induce significant levels of cytokines, and complementation of the asnH mutant with a plasmid expressing intact AsnH restored the cytokine production comparable to that of the wild-type strain (Fig. 2).
AsnH is an asparagine synthetase with glutamine amidotransferase activity asnH (1,878 bp) of L. casei ATCC 27139 encodes a 625-amino acid product with a predicted molecular mass of 73 kDa. A homology search determined that the asnH product has significant homology to the LtsA/AsnB glutamine amidotransferase family of proteins that have been identified in various Gram-positive and Gram-negative bacteria. The glutamine amidotransferase family includes proteins composed of an N-terminal glutaminase domain and a C-terminal synthetase domain with conserved amino acid motifs [20,21]. In AsnH of L. casei ATCC 27139, amino acid residues Cys-2, Arg-48, Asn-73, Glu-75, and Asp-97, which are essential for glutaminase activity of the N-terminal domain, and amino acid residues Ser-261, Asp-265, Ser-266, Gly-355, Asp-359, Lys-525, and Lys-545, which are required for catalytic activity of the C-terminal domain, are invariant (Fig. 3A) [20,[22][23][24].
To determine whether AsnH possess glutamine amidotransferase activity, we conducted an in vitro glutamic acid production assay. Glutaminase activity can be enhanced by the addition of an amide acceptor such as aspartic acid for E. coli AsnB or lysozymetreated cell wall extracts for Rhodococcus erythropolis LtsA [20]. Incubation of the purified AsnH WT -FLAG fusion proteins with glutamine resulted in glutamic acid production at a rate of 6.6 mM/h when lysozyme-treated cell wall extracts of L. casei ATCC 27139, but not aspartic acid, was added in the reaction  (Fig. 3B). To further characterize the AsnH as a glutamine amidotransferase, we used site-directed mutagenesis to replace the conserved N-terminal Cys-2 with Ser-2 and the conserved Cterminal Asp-265, which is located in the putative ATP-binding pocket of the synthetase domain, with Asn-265. The AsnH C2S -FLAG and AsnH D265N -FLAG mutant proteins failed to produce glutamic acid (Fig. 3B). In AsnB of E. coli, ATP and aspartic acid form a catalytic intermediate and NH 3 is transferred to the amide acceptor [21]. To test whether the enzymatic activity of AsnH of L. casei is enhanced by ATP hydrolysis, a non-hydrolyzable ATP analog, AMP-PNP [adenosine 59-(bc-imido) triphosphate], was used instead of ATP in the reaction. No glutamic acid production was detected in the AMP-PNP reaction mixture (Fig. 3B).

Structural analysis of the asnH mutant cell wall
AsnH of Lactococcus lactis and LtsA of R. erythropolis are involved in cell wall biosynthesis, and the mutations in asnH or ltsA confer increased bacterial sensitivity to lysozyme [20,25]. L. casei wildtype and asnH-complemented mutant strains were stained Gram positive, while the asnH mutant (MT77) was stained Gram negative (Fig. 4A). TEM observations of L. casei cells showed that the peptidoglycan layers of the mutant cells were significantly thinner (Fig. 4BC) and the cell size appeared to be larger when compared with those of the wild-type and the complemented cells (Fig. 4B).
In L. casei, the peptidoglycan stem peptide is composed of the tetrapeptide chain containing L-Ala-D-Glu-D-Lys-D-Ala, which is cross-linked with a D-Asp residue (Fig. 5) [26]. To evaluate the effect of asnH mutation on the cell wall structure, we analyzed the amino acid composition of the peptidoglycan layers of the L. casei cells. The molar ratio of Asp in the peptidoglycans extracted from the asnH mutant strain was lower than that of extracts from the wild-type and the complemented strains ( Table 2).
The lysozyme MIC of the asnH mutant (MT77) was 80 mg/ml, which is far lower than that of the wild-type strain as: .10,000 mg/ml ( Table 2). The asnH-complemented strain displayed a lysozyme resistance comparable to the wild-type strain ( Table 2). The vancomycin MIC of the asnH mutant was 8-fold lower than that of the wild-type and the complemented strains (data not shown).

Identification of the mutated region of MNNG-induced J1 phage-resistant mutants
We previously demonstrated that J1 phage-resistant mutants, which were obtained by chemical mutagenization of L. casei ATCC 27139 with N-methyl-N9-nitro-N-nitrosoguanidine (MNNG), exhibited the lower immune-augmenting activity [27]. To further clarify that AsnH is implicated in the activity, we cloned asnH from the MNNG-induced J1 phage-resistant mutants (strains 27139-J1R1, 27139-J1R2, 27139-J1R3, and 27139-J1R4). The mutation sites in the genes were found to be either a deletion (C-1207 deletion in 27139-J1R1) or displacement (G-788 to A-788 in J1R2, G-1486 to A-1486 in J1R3, and G-88 to A-88 in J1R4) of a base in asnH, resulting in frameshift (J1R1) or missense mutations (Gly-263 to Glu-263 in J1R2, Glu-496 to Lys-496 in J1R3, and Gly-30 to Ser-30 in J1R4) of AsnH (Fig. 6). These mutated residues are among the evolutionarily conserved amino acids essential for enzymatic activity of members of the LtsA/AsnB glutamine amidotransferase family (Fig. 6). Introducing a plasmid harboring asnH into the MNNG-induced J1 phage-resistant mutant strains recovered the J1 phage-sensitive phenotype (Table 3) and restored the immunoprotective effects associated with Listeria infection in mice (data not shown).

Discussion
Heat-killed L. casei ATCC 27139 significantly augments innate immunity in mice [16,27]. This immunoprotective effect is lost in J1 phage-resistant mutants [16,27], suggesting that certain cell wall components associated with J1 phage sensitivity are involved in the activation of host innate immunity. In this study, we used a Tn5 insertion library to demonstrate that asnH, dnaJ, and dnaK are coordinated with J1 phage sensitivity, and only asnH mutants lost the ability to enhance host innate immunity. Complementation of  the asnH mutant strains with the cloned asnH recovered the activity. MNNG-induced J1 phage-resistant mutants lacking the capacity to augment innate immunity all had mutated asnH, reinforcing the idea that asnH is essential for the activity of L. casei ATCC 27139 to boost host innate immunity. DnaJ and DnaK proteins are molecular chaperones that regulate protein folding and function as heat shock proteins [28]. Because the dnaJ and dnaK mutants of L. casei ATCC 27139 displayed anti-listerial activity equivalent to the wild-type strain, it is unlikely that the dnaJ or dnaK gene contributes to the immuneaugmenting activity. Loss of innate immunity-augmenting activity in J1 phage-resistant mutants does not result simply from the phage resistance but from a specific phenomenon related to the loss of AsnH activity.
Asparagine synthetase, which consists of glutaminase activity and synthetase activity, catalyzes asparagine and glutamic acid biosynthesis from aspartic acid and glutamine, respectively [29,30]. The synthetase activity of the C-terminal domain recognizes an amide donor and forms an intermediate before the glutaminase activity of the N-terminal domain hydrolyzes an amide donor, and this involves an ATP-dependent transfer of ammonia to aspartic acid yielding asparagine in the presence of magnesium ion [31]. Although glutamine-hydrolyzing AsnB of several bacteria utilizes glutamine as an amide donor [32,33] and glutaminase activity is markedly enhanced when the amide acceptor aspartic acid is added in the reaction mixture [24], glutaminase activity of R. erythropolis LtsA is enhanced significantly when lysozyme-treated cell wall extracts are added instead of aspartic acid in the reaction mixture [20]. In the present study, L. casei ATCC 27139 AsnH displayed marked glutaminase activity when the lysozyme-treated cell wall extracts of ATCC 27139 were added instead of aspartic acid, strongly suggesting that components of the lysozyme-treated cell wall extracts serve as amide acceptors. L. lactis AsnH, which exhibits 59% amino acid sequence identity with the L. casei AsnH, is involved in amidation of D-Asp present in the interpeptide cross-bridge of peptidoglycan (Fig. 5) [25]. In the maturation of L. lactis peptidoglycan, approximately 75% of the side chain and cross-bridge residues are amidated, indicating that D-Asp is converted to D-Asn [34]. Homologous genes have been identified in other Gram-positive bacterial species that possess D-Asn in their cross-bridges, and L. casei peptidoglycan also possesses D-Asn in its cross-bridges [35]. In this study, the assays of the asnH-mutant cells about lysozyme sensitivity, Gram staining, and TEM observations showed the lack of the thick and rigid peptidoglycan features that are characteristic to the wild-type cells, indicating that AsnH is required for the synthesis of intact peptidoglycans. Sequence analysis by SignalP [36] indicates that AsnH contains neither a putative signal peptide nor a transmembrane segment, suggesting that AsnH is localized inside the bacterial cytoplasm and that this protein most probably acts on peptidoglycan precursors. Although the analysis of amino acid compositions in peptidoglycan of the asnH mutant cells showed a decrease in aspartic acid content, further experiments would be needed to elucidate where AsnH protein acts on the peptidoglycan. Peptidoglycan and derived muropeptides in L. salivarius showed protective effect in murine colitis mice model through induction of pathogen-associated molecular pattern receptors such as Nod2 [37], which recognizes intracellular muramyl dipeptide of a peptidoglycan constituent [38], suggesting the relevance of peptidoglycan structure to the immune-augmenting activity of L. casei ATCC 27139.
On the other hand, the changed amino acid compositions in peptidoglycan may affect the immune signaling by non-peptidoglycan molecules. Cell surface polysaccharide components, Dgalactosamine and L-rhamnose, in L. casei ATCC 27139/S-1 comprise a phage receptor for J1 phage, and J1 phage-resistant mutant lacked D-galactosamine in its surface components [39]. In this study, although no significant difference in the polysaccharide thickness between the wild-type and the asnH mutant cells has been identified (data not shown), the amount of polysaccharide in the asnH mutant cells appeared to be less organized. In L. casei strain Shirota, polysaccharide-peptidoglycan complexes play important roles in augmenting host innate immunity [7,40], which, taken together, suggests the relevance of cell surface polysaccharide components to the immune-activating capacity of L. casei ATCC 27139. Teichoic acids in L. plantarum has been shown to modulate intestinal and systemic immune responses in a TLR2-dependent manner [41]. TLR2 recognizes bacterial components such as lipoteichoic acid, lipoprotein [42,43], LPS [44,45], the mycobacterial lipoarabinomannan [46], and  heat-killed Gram-positive bacteria [47]. L. casei ATCC 27139-J1R1, asnH mutant, lost the capacity to induce TLR2 and Nod2 [16]. Demonstration of the differences in the amount of cell wall components between the wild-type and the asnH mutant cells might lead to further elucidation of the components and structures that enhance host innate immunity.
In conclusion, asnH of the probiotic L. casei ATCC 27139 is suggested to be involved in the immune-activating capacity of this strain. asnH contributes to peptide synthesis in the peptidoglycan layer, indicating that certain cell wall structures of L. casei are important in the enhancement of host innate immunity. These findings should facilitate the characterization of active components and structures in probiotic lactobacilli to augment host innate immunity.