Deficiency of G protein‐coupled receptor <i>Gpr111/Adgrf2</i> causes enamel hypomineralization in mice by alteration of the expression of kallikrein‐related peptidase 4 (<i>Klk4</i>) during <scp>pH</scp> cycling process

Chiba, Yuta; Yoshizaki, Keigo; Satô, Hiroshi; Ikeuchi, Tomoko; Rhodes, Craig; Chiba, Mitsuki; Saito, Kan; Nakamura, Takashi; Iwamoto, Tsutomu; Yamada, Aya; Yamada, Yoshihiko; Fukumoto, Satoshi

doi:10.1096/fj.202202053r

Cited by 2 publications

(3 citation statements)

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“…Matrices such as Ambn and Amelx are important for the initiation of calcification, whereas enzymes such as Klk4 are important for hypercalcification. Therefore, an appropriate dose of protease is essential for enamel formation, and deficiency or excess of Klk4 causes enamel dysplasia 8,66 . In the present study, Ambn , Amelx , and Klk4 were upregulated during ameloblast differentiation; however, S100a6 knockdown suppressed Ambn and Amelx expression (Figure 5A).…”

Section: Discussionsupporting

confidence: 44%

“…(A) (B) dysplasia. 8,66 In the present study, Ambn, Amelx, and Klk4 were upregulated during ameloblast differentiation; however, S100a6 knockdown suppressed Ambn and Amelx expression (Figure 5A). The suppression of Ambn and Amelx suggests that the loss of S100a6 inhibited the difof ameloblasts.…”

Section: (A) (B) (C)mentioning

confidence: 40%

“…[4][5][6][7] Calcification is performed using the enamel matrix as a scaffold, 4,5 which is later degraded by proteases such as matrix metalloproteinase-20 and kallikrein-related peptidase 4 (Klk4) to enhance calcification. Although extensive studies have been performed on the differentiation of the dental epithelium into mature ameloblasts, 8,9 the calcification process remains poorly understood.…”

Section: Introductionmentioning

confidence: 99%

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S100a6 knockdown promotes the differentiation of dental epithelial cells toward the epidermal lineage instead of the odontogenic lineage

Otake,

Saito,

Chiba

et al. 2024

The FASEB Journal

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Tooth development is a complex process involving various signaling pathways and genes. Recent findings suggest that ion channels and transporters, including the S100 family of calcium‐binding proteins, may be involved in tooth formation. However, our knowledge in this regard is limited. Therefore, this study aimed to investigate the expression of S100 family members and their functions during tooth formation. Tooth germs were extracted from the embryonic and post‐natal mice and the expression of S100a6 was examined. Additionally, the effects of S100a6 knockdown and calcium treatment on S100a6 expression and the proliferation of SF2 cells were examined. Microarrays and single‐cell RNA‐sequencing indicated that S100a6 was highly expressed in ameloblasts. Immunostaining of mouse tooth germs showed that S100a6 was expressed in ameloblasts but not in the undifferentiated dental epithelium. Additionally, S100a6 was localized to the calcification‐forming side in enamel‐forming ameloblasts. Moreover, siRNA‐mediated S100a6 knockdown in ameloblasts reduced intracellular calcium concentration and the expression of ameloblast marker genes, indicating that S100a6 is associated with ameloblast differentiation. Furthermore, S100a6 knockdown inhibited the ERK/PI3K signaling pathway, suppressed ameloblast proliferation, and promoted the differentiation of the dental epithelium toward epidermal lineage. Conclusively, S100a6 knockdown in the dental epithelium suppresses cell proliferation via calcium and intracellular signaling and promotes differentiation of the dental epithelium toward the epidermal lineage.

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Section: Discussionsupporting

confidence: 44%

Section: (A) (B) (C)mentioning

confidence: 40%