The complex formation of MASP-3 with pattern recognition molecules of the lectin complement pathway retains MASP-3 in the circulation

Kohei Kusakari; Takeshi Machida; Yumi Ishida; Tomoko Omori; Toshiyuki Suzuki; Masayuki Sekimata; Ikuo Wada; Teizo Fujita; Hideharu Sekine

doi:10.3389/fimmu.2022.907023

The complex formation of MASP-3 with pattern recognition molecules of the lectin complement pathway retains MASP-3 in the circulation

Front Immunol. 2022 Aug 16:13:907023. doi: 10.3389/fimmu.2022.907023. eCollection 2022.

Authors

Kohei Kusakari¹, Takeshi Machida¹, Yumi Ishida¹, Tomoko Omori¹, Toshiyuki Suzuki², Masayuki Sekimata², Ikuo Wada³, Teizo Fujita⁴, Hideharu Sekine¹

Affiliations

¹ Department of Immunology, Fukushima Medical University, Fukushima, Japan.
² Radioisotope Research Center, Fukushima Medical University, Fukushima, Japan.
³ Department of Cell Science, Institute of Biomedical Sciences, Fukushima Medical University, Fukushima, Japan.
⁴ Fukushima Prefectural General Hygiene Institute, Fukushima, Japan.

Abstract

The complement system plays an important role in host defense and is activated via three different activation pathways. We have previously reported that mannose-binding lectin-associated serine protease (MASP)-3, unlike its splicing variant MASP-1, circulates in an active form and is essential for the activation of the alternative pathway (AP) via the activation of complement factor D (FD). On the other hand, like MASP-1 and MASP-2 of the lectin pathway (LP), MASP-3 forms a complex with the pattern recognition molecules (PRMs) of the LP (LP-PRMs). Both MASP-1 and MASP-2 can be activated efficiently when the LP-PRMs complexed with them bind to their ligands. On the other hand, it remains unclear how MASP-3 is activated, or whether complex formation of MASP-3 with LP-PRMs is involved in activation of MASP-3 or its efficiency in the circulation. To address these issues, we generated wild-type (WT) and four mutant recombinant mouse MASP-3 proteins fused with PA (human podoplanin dodecapeptide)-tag (rmMASP-3-PAs), the latter of which have single amino acid substitution for alanine in the CUB1 or CUB2 domain responsible for binding to LP-PRMs. The mutant rmMASP-3-PAs showed significantly reduced in-vivo complex formation with LP-PRMs when compared with WT rmMASP-3-PA. In the in-vivo kinetic analysis of MASP-3 activation, both WT and mutant rmMASP-3-PAs were cleaved into the active forms as early as 30 minutes in the circulation of mice, and no significant difference in the efficiency of MASP-3 cleavage was observed throughout an observation period of 48 hours after intravenous administration. All sera collected 3 hours after administration of each rmMASP-3-PA showed full restoration of the active FD and AP activity in MASP-3-deficient mouse sera at the same levels as WT mouse sera. Unexpectedly, all mutant rmMASP-3-PAs showed faster clearance from the circulation than the WT rmMASP-3-PA. To our knowledge, the current study is the first to show in-vivo kinetics of MASP-3 demonstrating rapid activation and clearance in the circulation. In conclusion, our results demonstrated that the complex formation of MASP-3 with LP-PRMs is not required for in-vivo activation of MASP-3 or its efficiency, but may contribute to the long-term retention of MASP-3 in the circulation.

Keywords: MASP-3; alternative pathway; complement; lectin pathway; pattern recognition molecules.

MeSH terms

Animals
Complement Pathway, Mannose-Binding Lectin* / physiology
Complement System Proteins
Humans
Kinetics
Lectins / genetics
Lectins / metabolism
Mannose-Binding Protein-Associated Serine Proteases* / genetics
Mannose-Binding Protein-Associated Serine Proteases* / metabolism
Mice
Mutation
Recombinant Proteins / metabolism

Substances

Lectins
Recombinant Proteins
Complement System Proteins
MASP-3 protein, mouse
Mannose-Binding Protein-Associated Serine Proteases