Ceramide kinase
In enzymology, a ceramide kinase, also abbreviated as CERK, is an enzyme that catalyzes the chemical reaction:
Thus, the two substrates of this enzyme are ATP and ceramide, whereas its two products are ADP and ceramide-1-phosphate.
This enzyme belongs to the family of transferases, specifically those transferring phosphorus-containing groups with an alcohol group as acceptor. The systematic name of this enzyme class is ATP:ceramide 1-phosphotransferase. This enzyme is also called acylsphingosine kinase. This enzyme participates in sphingolipid metabolism.
Gene
CERK is encoded by the CERK gene. The CERK gene is located on human chromosome 22q13, contains 13 exons, and is approximately 4.5kb in length. CERK shares sequence homology with sphingosine kinase type I, including an N-terminal pleckstrin homology domain and a diacylglycerol kinase domain. BLAST searches of expressed sequence tag by Sugiura and colleagues have yielded results showing orthologous CERK genes in other eukaryotes including Drosophila melanogaster, Caenorhabditis elegans, and Oryza sativa. A mouse homolog has been cloned as well.The complete gene of human CERK contains 4459bp, which consists of a 123bp-5’-untranslated region, a 2772bp 3’-non-coding, and a 1611bp open reading frame. Sequence analysis of CERK putatively suggests that the following post-translational modification sites exist: 4 N-glycosylation sites, 15 phosphorylation sites, 5 prenylation sites, and 2 amidation sites. The complete gene of mouse CERK differed slightly, containing a 1593bp open reading frame. The decreased length of the open reading frame results in the loss of 2 prenylation sites and 1 amidation site.
In human CERK, a retinoic acid response element -like exists between -40bp and -28bp and contains the sequence: TCCCCG C CGCCCG. RARE-like plays a role in transcription regulation of CERK. It is suspected that in the presence of all-trans retinoic acid, transcription factor">transcriptional">transcription factor I, retinoic acid receptor, retinoid X receptor bind the RARE-like of CERK in 5H-SY5Y cells. However, CERK expression varies per cell line. In contrast to SH-SY5Y neuroblastoma cells, HL60 leukemia cells demonstrated no binding of CERK even in the presence of ATRA. This suggests that differential expression of RARα, RXRα, and COUP-PTI may determine transcription levels in various cell lines.
Protein
CERK is a 537 amino acid enzyme in humans. CERK was first discovered in 1989 when it was co-purified with synaptic vesicles from brain cells. Upon discovery, CERK was proposed to be a ceramide kinase that functions in the presence of μM concentration of calcium anions. Since CERK lacks a calcium binding site, the regulatory mechanism of CERK was poorly understood. CERK was later confirmed to bind calmodulin in the presence of calcium, indicating the calmodulin first binds calcium and then CERK. Once bound, CERK becomes active and is capable of phosphorylating ceramides. Binding of calmodulin occurs between amino acids 420 and 437 in CERK at a putative 1-8-14B calmodulin binding motif. The binding motif in CERK contains leu-422, phe-429, and leu-435 which respectively correspond to the 1st, 8th, and 14th hydrophobic amino acids where calmodulin binds. Mutation of Phe-429 results in weak calmodulin binding, while mutations of Phe-331 or Phe-335 entirely preclude binding.CERK activity has primarily been observed within human neutrophils, cerebrum granule cells, and epithelium-derived lung cells. When inactive, CERK is suspended within the cytosol of the cell. When CERK is activated by interleukin-1β, it is localized to the trans-golgi, and from there, possibly delivered to the plasma membrane. Activation may also to cause CERK to localize within endosomes. CERK’s PH domain plays an integral role in this localization. Once localized, to the trans-golgi CERK activates cytosolic phospholipase A2 that has localized to the trans-golgi. Activation of cPLA2 results in hydrolysis of membrane phospholipids to produce arachidonic acid. Ceramide kinase has also been demonstrated to regulate localization and level of phosphatidylinositol 4,5-bisphosphate produced from NORPA, a phospholipase C homolog in Drosophila melanogaster. In addition to endosomal and trans-golgi localization, CERK has been found to localize to outer mitochondrial membrane at the site of COX-2 localization in A549 cells.