Cervicale alae of head of Toxocara cati
Cephalic alae of head of Enterobius vermicularis (human pinworm)
18: Lateral view of caudal bursa, showing projections supported by bursal rays.

The alae is a protruding ridge that forms longitudinally on many nematodes. In the Caenorhabditis elegans nematode they are present in the L1, dauer (an alternative long living larvae stage where the nematode is dormant) and adult stages. The alae are most pronounced during the dauer larval stage and not present in the L2, and L3 C. elegans stages.

The term ‘alae’ is the plural of ala (wing), describing either one of the pair of ridges that forms on a nematode or an individual crease found on an individual ridge. The term ‘ala’ is rarely used in describing the alae and scientific journals use the term ‘alae’ both singularly and in the plural.

Structure

The alae is formed by the hypodermal seam cells where a fibrous ribbon of a zona pellucida (ZP) domain protein is produced. In C. elegans many of these proteins are termed CUT-1.[1] The CUT refers to cuticulins which are the various proteins that are not solubilised by both reducing agents and detergents[2] made insoluble by the nature of their crosslinks.[3][4]

Described as a matrix that appears to be holding the two sides of the collagenous cuticle together for strengthening[5] it should also be interpreted as a matrix separating the cuticle thereby exposing itself to the external environment.[6] The alae is formed during an oxidative process where peroxidase acts on protein bound tyrosine residues. The alae is a crease, that by the cross linking process causes radial shrinking of the seam cell secreted proteins.

Function

The function of the alae is not yet clear. It is generally given a function related to cuticle strength, nematode movement or fat storage. But the predominant structure of the C. elegans alae contain the ZP domain proteins (CUT-1, CUT-3, CUT-5). The ZP domain had been termed ‘the sequence in search of a function’ and has been given the functional role of matrix assembly and also putatively, functions in pheromone and olfactory signal transduction.[7][8] Despite the structural nature of the ZP domain, it is not the ideal protein for strength alone. Wherever ZP domains are found, they are found in definite or putative association with signal transduction accompanied by interaction with an external or hostile environment.

Function based on genetic data of the H. Contortus dauer nematode

In the parasitic nematode Haemonchus contortus a ZP domain protein of a dauer stage nematode has been genetically associated to a target molecule found in the environment that this nematode could be using for exiting the dauer stage. This was statistically related with a high degree of significance indicating that the alae may specifically function as a receptor site.

In the case of H. contortus the dauer nematode can remain in the gastric epithelium for months and until the right signals indicating conditions outside the host are favorable for egg survival, it will then trigger resumption of development. During the dauer stage the mouth and anal openings are sealed and neural receptors around the head retracted. The alae is more pronounced than at any other stage and remains exposed to the external environment. Triggers for exiting the dauer state may be determined by the concentration of target molecules around the nematode. In order to measure concentrations accurately, a very large receptor area is necessary, hence a structure such as the alae may be required.

Postulated function

The alae appears to be a neural receptor responsive to just a handful of molecules particular to each species of nematode. Up to half a dozen types of receptors may be present at any one time on the alae and each type would be very numerous. The target molecules in the environment that stimulate each type of receptor may then be measured for their concentration and a threshold reached before an action is instigated. These actions may instigate entry into the dauer state (L1 alae), exiting of the dauer state (pheromone and or presence of an indicator for food availability), for sexual reproduction where the area around the vulva and gonads of the female and male use this family of receptors (RAM-5) where the nematode is likely to identify that reproductive organs are in contact.[9] And quite probably there are some other functions that we have not yet been found.

References

  1. Ristoratore, F; Cermola, M; Nola, M; Bazzicalupo, P; Favre, R (July 1994). "Ultrastructural immuno-localization of CUT-1 and CUT-2 antigenic sites in the cuticles of the nematode Caenorhabditis elegans". Journal of Submicroscopic Cytology and Pathology. 26 (3): 437–43. PMID 8087805.
  2. Fujimoto, Daisaburo; Kanaya, Shigenori (July 1973). "Cuticlin: a noncollagen structural protein from Ascaris cuticle". Archives of Biochemistry and Biophysics. 157 (1): 1–6. doi:10.1016/0003-9861(73)90382-2. PMID 4352055.
  3. Lewis, E.; Sebastiano, M.; Nola, M.; Zei, F.; Lassandro, F.; Ristoratore, F.; Cermola, M.; Favre, R.; Bazzicalupo, P. (1 October 2014). "Cuticlin genes of nematodes". Parasite. 1 (1S): S57–S58. doi:10.1051/parasite/199401s1057.
  4. Lewis, E; Hunter, SJ; Tetley, L; Nunes, CP; Bazzicalupo, P; Devaney, E (25 June 1999). "cut-1-like genes are present in the filarial nematodes, Brugia pahangi and Brugia malayi, and, as in other nematodes, code for components of the cuticle". Molecular and Biochemical Parasitology. 101 (1–2): 173–83. doi:10.1016/S0166-6851(99)00070-5. PMID 10413052.
  5. De Giorgi, C.; De Luca, F.; Di Vito, M.; Lamberti, F. (20 February 1997). "Modulation of expression at the level of splicing of cut-1 RNA in the infective second-stage juvenile of the plant parasitic nematode Meloidogyne artiellia". Molecular and General Genetics. 253 (5): 589–598. doi:10.1007/s004380050361. PMID 9065692. S2CID 11819745.
  6. Vermont, R.C., (2003) Characterisation of cDNA from Haemonchus contortus (Barber's pole worm) encoding a Cuticulin. Dissertation, Charles Sturt University NSW. This information is not publicly available and is held at CSU School of Agriculture. Further information may be sourced by emailing the author
  7. Matsushita, F; Miyawaki, A; Mikoshiba, K (16 February 2000). "Vomeroglandin/CRP-Ductin is strongly expressed in the glands associated with the mouse vomeronasal organ: identification and characterization of mouse vomeroglandin". Biochemical and Biophysical Research Communications. 268 (2): 275–81. doi:10.1006/bbrc.2000.2104. PMID 10679193.
  8. Sutton, KA; Jungnickel, MK; Florman, HM (June 2002). "If music be the food of love…". Nature Cell Biology. 4 (6): E154-5. doi:10.1038/ncb0602-e154. PMID 12042831. S2CID 42749251.
  9. Yu, RY; Nguyen, CQ; Hall, DH; Chow, KL (17 July 2000). "Expression of ram-5 in the structural cell is required for sensory ray morphogenesis in Caenorhabditis elegans male tail". The EMBO Journal. 19 (14): 3542–55. doi:10.1093/emboj/19.14.3542. PMC 313976. PMID 10899109.
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