In this communication we present a method for single-slice mapping of ultrashort transverse relaxation times T(2). The RF pulse sequence consists of a spin echo preparation of the magnetization followed by slice-selective ultrashort echo time (UTE) imaging with radial k-space sampling. In order to keep the minimum echo time as small as possible, avoid out-of-slice contamination and signal contamination due to unwanted echoes, the implemented pulse sequence employs a slice-selective 180° RF refocusing pulse and a 4-step phase cycle. The slice overlap of the two slice-selective RF pulses was investigated. An acceptable Gaussian slice profile could be achieved by adjusting the strength of the two slice-selection gradients. The method was tested on a short T(2) phantom consisting of an arrangement of a roll of adhesive tape, an eraser, a piece of modeling dough made of Plasticine®, and a 10% w/w agar gel. The T(2) measurements on the phantom revealed exponential signal decays for all samples with T(2)(adhesive tape)=(0.5 ± 0.1)ms, T(2)(eraser)=(2.33 ± 0.07)ms, T(2)(Plasticine®)=(2.8 ± 0.06)ms, and T(2)(10%agar)=(9.5 ± 0.83)ms. The T(2) values obtained by the mapping method show good agreement with the T(2) values obtained by a non-selective T(2) measurement. For all samples, except the adhesive tape, the effective transverse relaxation time T(2)(∗) was significantly shorter than T(2). Depending on the scanner hardware the presented method allows mapping of T(2) down to a few hundreds of microseconds. Besides investigating material samples, the presented method can be used to study the rapidly decaying MR-signal from biological tissue (e.g.: bone, cartilage, and tendon) and quadrupolar nuclei (e.g.: (23)Na, (35)Cl, and (17)O).
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