Characterization and expression analysis of the yellow lupin (Lupinus luteus L.) gene coding for nodule specific proline-rich protein

Abstract

The LIPRP2 gene coding for a proline-rich protein shows a high level of similarity to, as well as significant differences from the family of ENOD2 nodule-specific genes. Several sequence motifs with putative regulatory function were identified in the 5′ and 3′ noncoding regions of the LIPRP2 gene. Northern blot analysis revealed that the expression of the LIPRP2 gene begins 9 days after inoculation of yellow lupin roots with Bradyrhizobium sp. (Lupinus); the expression is restricted to symbiotic nodules and is not detected in other tissues or organs. Detailed hybridization analysis showed that, when expression is activated, the LIPRP2 transcript is modified so as to produce at least three bands and a continuous distribution of decay intermediates. The modification of the LIPRP2 transcript probably involves degradation from the 5′-and/or 3′-ends of the RNA molecules. Southern blot analysis indicates that only one gene is present in the yellow lupin genome. The presence of genes homologous to the LIPRP2 gene was confirmed for three cultivars of yellow lupin and for Lupinus angustifolius. However, LIPRP2 homologues were not detected in Lupinus albus cv. Bac, indicating that this plant may lack the ENOD2 sequence.